| Literature DB >> 22051800 |
Magdalena Harakalova1, Michal Mokry, Barbara Hrdlickova, Ivo Renkens, Karen Duran, Henk van Roekel, Nico Lansu, Mark van Roosmalen, Ewart de Bruijn, Isaac J Nijman, Wigard P Kloosterman, Edwin Cuppen.
Abstract
The unprecedented increase in the throughput of DNA sequencing driven by next-generation technologies now allows efficient analysis of the complete protein-coding regions of genomes (exomes) for multiple samples in a single sequencing run. However, sample preparation and targeted enrichment of multiple samples has become a rate-limiting and costly step in high-throughput genetic analysis. Here we present an efficient protocol for parallel library preparation and targeted enrichment of pooled multiplexed bar-coded samples. The procedure is compatible with microarray-based and solution-based capture approaches. The high flexibility of this method allows multiplexing of 3-5 samples for whole-exome experiments, 20 samples for targeted footprints of 5 Mb and 96 samples for targeted footprints of 0.4 Mb. From library preparation to post-enrichment amplification, including hybridization time, the protocol takes 5-6 d for array-based enrichment and 3-4 d for solution-based enrichment. Our method provides a cost-effective approach for a broad range of applications, including targeted resequencing of large sample collections (e.g., follow-up genome-wide association studies), and whole-exome or custom mini-genome sequencing projects. This protocol gives details for a single-tube procedure, but scaling to a manual or automated 96-well plate format is possible and discussed.Mesh:
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Year: 2011 PMID: 22051800 DOI: 10.1038/nprot.2011.396
Source DB: PubMed Journal: Nat Protoc ISSN: 1750-2799 Impact factor: 13.491