2013
DOI: 10.1016/j.gene.2013.07.040
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Emulsion PCR-coupled target enrichment: An effective fishing method for high-throughput sequencing of poorly preserved ancient DNA

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Cited by 19 publications
(10 citation statements)
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“…However, it is difficult to rule out inter-locus amplification bias as the origin of this pattern; only two samples (Mammoths 9 and 10) show low correlations between regional duplication rate and unique coverage depth, and for these samples unique enrichment rates do not correspond to bait properties. That amplification biases appear to dictate coverage patterns in this data set clearly encourages the use of amplification-minimal techniques (15, 42, 43) with less biased DNA polymerases (40, 44) or emulsion PCR (45). …”
Section: Resultsmentioning
confidence: 68%
“…However, it is difficult to rule out inter-locus amplification bias as the origin of this pattern; only two samples (Mammoths 9 and 10) show low correlations between regional duplication rate and unique coverage depth, and for these samples unique enrichment rates do not correspond to bait properties. That amplification biases appear to dictate coverage patterns in this data set clearly encourages the use of amplification-minimal techniques (15, 42, 43) with less biased DNA polymerases (40, 44) or emulsion PCR (45). …”
Section: Resultsmentioning
confidence: 68%
“…The first genetic marker analyzed in human paleogenetic studies was mitochondrial DNA (mtDNA) because of its higher copy number in the cell than nuclear DNA. Probe hybridization assays used biotinylated DNA or RNA probes targeting the two hypervariable segments of the mtDNA control region (CR) ( Briggs et al, 2009 ; Krause et al, 2010 ; Maricic et al, 2010 ; Enk et al, 2013 ; Kihana et al, 2013 ; Templeton et al, 2013 ; Eduardoff et al, 2017 ; Loreille et al, 2018 ). Another uniparental marker, the Y-chromosome DNA (Y-DNA), was also used to study aDNA.…”
Section: Early Developments Of Hybrid-capture Strategies: Human Genetmentioning
confidence: 99%
“…The rise of MPS-based assays significantly increased the success of obtaining useful genetic data from ancient specimens [ 16 , 17 ], especially by using DNA hybridization enrichment and single-step PCR primer extension capture (PEC) [ 18 ]. Probe hybridization assays use 70–500 base pair (bp)-long biotinylated DNA or RNA probes hybridizing to regions in the mitogenome, and are either generated from PCR products [ 19 , 20 , 21 , 22 ] or designed and made commercially available (e.g., Mybaits (Microarray, Ann Arbor, MI, USA) [ 23 ] or Agilent’s SureSelect (Agilent Technologies, Santa Clara, CA, USA) [ 24 ]). However, the protocols usually require high library DNA input (more than 100 ng), and the hybridization steps can take up to 72 h. Single Step Extension Capture was developed by Briggs et al in 2009 [ 25 ] for the sequence analysis of Neanderthal mitogenomes.…”
Section: Introductionmentioning
confidence: 99%