From micrograms to picograms: quantitative PCR reduces the material demands of high-throughput sequencing
Author(s) -
Matthias Meyer,
Adrian W. Briggs,
Tomislav Maričić,
Barbara Höber,
Barbara Höffner,
Johannes Krause,
Antje Weihmann,
Svante Pääbo,
Michael Hofreiter
Publication year - 2007
Publication title -
nucleic acids research
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 9.008
H-Index - 537
eISSN - 1362-4954
pISSN - 0305-1048
DOI - 10.1093/nar/gkm1095
Subject(s) - biology , pyrosequencing , dna sequencing , deep sequencing , computational biology , illumina dye sequencing , polymerase chain reaction , genome , shotgun sequencing , genomic dna , genetics , dna , gene
Current efforts to recover the Neandertal and mammoth genomes by 454 DNA sequencing demonstrate the sensitivity of this technology. However, routine 454 sequencing applications still require microgram quantities of initial material. This is due to a lack of effective methods for quantifying 454 sequencing libraries, necessitating expensive and labour-intensive procedures when sequencing ancient DNA and other poor DNA samples. Here we report a 454 sequencing library quantification method based on quantitative PCR that effectively eliminates these limitations. We estimated both the molecule numbers and the fragment size distributions in sequencing libraries derived from Neandertal DNA extracts, SAGE ditags and bonobo genomic DNA, obtaining optimal sequencing yields without performing any titration runs. Using this method, 454 sequencing can routinely be performed from as little as 50 pg of initial material without titration runs, thereby drastically reducing costs while increasing the scope of sample throughput and protocol development on the 454 platform. The method should also apply to Illumina/Solexa and ABI/SOLiD sequencing, and should therefore help to widen the accessibility of all three platforms.
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