Abstract

Single nucleotide polymorphism (SNP) discovery and genotyping are essential to genetic mapping. There remains a need for a simple, inexpensive platform that allows high-density SNP discovery and genotyping in large populations. Here we describe the sequencing of restriction-site associated DNA (RAD) tags, which identified more than 13,000 SNPs, and mapped three traits in two model organisms, using less than half the capacity of one Illumina sequencing run. We demonstrated that different marker densities can be attained by choice of restriction enzyme. Furthermore, we developed a barcoding system for sample multiplexing and fine mapped the genetic basis of lateral plate armor loss in threespine stickleback by identifying recombinant breakpoints in F(2) individuals. Barcoding also facilitated mapping of a second trait, a reduction of pelvic structure, by in silico re-sorting of individuals. To further demonstrate the ease of the RAD sequencing approach we identified polymorphic markers and mapped an induced mutation in Neurospora crassa. Sequencing of RAD markers is an integrated platform for SNP discovery and genotyping. This approach should be widely applicable to genetic mapping in a variety of organisms.

Keywords

BiologyMolecular Inversion ProbeGenotypingGeneticsSNP genotypingSingle-nucleotide polymorphismComputational biologySNPTag SNPGenotypeGene

Affiliated Institutions

Related Publications

Publication Info

Year
2008
Type
article
Volume
3
Issue
10
Pages
e3376-e3376
Citations
3432
Access
Closed

External Links

View on DOI.org

Social Impact

Altmetric
PlumX Metrics

Social media, news, blog, policy document mentions

Citation Metrics

3432
OpenAlex

Cite This

Nathan A. Baird, Paul D. Etter, Tressa S. Atwood et al. (2008). Rapid SNP Discovery and Genetic Mapping Using Sequenced RAD Markers. PLoS ONE , 3 (10) , e3376-e3376. https://doi.org/10.1371/journal.pone.0003376

Identifiers

DOI
10.1371/journal.pone.0003376