Effective BAC clone anchoring with genotyping-by-sequencing and diversity arrays technology in a large genome cereal rye.
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Identifcation of bacterial artifcial chromosome (BAC) clones containing specifc sequences is a prerequisite for many applications, such as physical map anchoring or gene cloning. Existing BAC library screening strategies are either low-throughput or require a considerable initial input of resources for platform establishment. We describe a high-throughput, reliable, and cost-efective BAC library screening approach deploying genotyping platforms which are independent from the availability of sequence information: a genotyping-by-sequencing (GBS) method DArTSeq and the microarray-based Diversity Arrays Technology (DArT). The performance of these methods was tested in a very large and complex rye genome. The DArTseq approach delivered superior results: a several fold higher efciency of addressing genetic markers to BAC clones and anchoring of BAC clones to genetic map and also a higher reliability. Considering the sequence independence of the platform, the DArTseq-based library screening can be proposed as an attractive method to speed up genomics research in resource poor species.
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Rekord utworzony: | 19 czerwca 2018 09:19 |
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Ostatnia aktualizacja: | 16 czerwca 2021 13:20 |