Abstract
Genome-wide molecular markers are often being used to evaluate genetic diversity in germplasm collections and for making genomic selections in breeding programs. To accurately predict phenotypes and assay genetic diversity, molecular markers should assay a representative sample of the polymorphisms in the population under study. Ascertainment bias arises when marker data is not obtained from a random sample of the polymorphisms in the population of interest. Genotyping-by-sequencing (GBS) is rapidly emerging as a low-cost genotyping platform, even for the large, complex, and polyploid wheat (Triticum aestivum L.) genome. With GBS, marker discovery and genotyping occur simultaneously, resulting in minimal ascertainment bias. The previous platform of choice for whole-genome genotyping in many species such as wheat was DArT (Diversity Array Technology) and has formed the basis of most of our knowledge about cereals genetic diversity. This study compared GBS and DArT marker platforms for measuring genetic diversity and genomic selection (GS) accuracy in elite U.S. soft winter wheat. From a set of 365 breeding lines, 38,412 single nucleotide polymorphism GBS markers were discovered and genotyped. The GBS SNPs gave a higher GS accuracy than 1,544 DArT markers on the same lines, despite 43.9% missing data. Using a bootstrap approach, we observed significantly more clustering of markers and ascertainment bias with DArT relative to GBS. The minor allele frequency distribution of GBS markers had a deficit of rare variants compared to DArT markers. Despite the ascertainment bias of the DArT markers, GS accuracy for three traits out of four was not significantly different when an equal number of markers were used for each platform. This suggests that the gain in accuracy observed using GBS compared to DArT markers was mainly due to a large increase in the number of markers available for the analysis.
Highlights
Genomic selection (GS) is a new marker assisted selection method based on the simultaneous use of whole-genome molecular markers to estimate breeding values for quantitative traits [1]
Lines were genotyped with 5,000 Diversity Array Technology (DArT) markers resulting in 1,544 polymorphic markers
Our results indicated that the DArT and GBS marker data yielded significantly different results for several statistics related to diversity
Summary
Genomic selection (GS) is a new marker assisted selection method based on the simultaneous use of whole-genome molecular markers to estimate breeding values for quantitative traits [1]. Reviews are available on the application of GS to plant breeding [3]. Key to implementing GS is the availability of inexpensive whole-genome genotyping. One such recently developed platform is Genotyping-by-Sequencing (GBS) [4]. Using advances in generation sequencing technologies, this approach uses sequencing of multiplexed, reduced-representation libraries constructed using restriction enzymes to obtain single nucleotide polymorphism (SNP) data. The multiplexed libraries are sequenced on a single run of a massively parallel sequencing platform. GBS typically generates a very large numbers of markers but with a high rate of missing data because genomic fragments in the library are sequenced at low depth leading to some fragments having zero coverage in some individuals
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