4.3 Article

A practical method for barcoding and size-trimming PCR templates for amplicon sequencing

BIOTECHNIQUES (2016)

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Journal

BIOTECHNIQUES
Volume 60, Issue 2, Pages 88-90

Publisher

BIOTECHNIQUES OFFICE
DOI: 10.2144/000114380

Keywords

next-generation sequencing; PCR; ligation; primer; polyclonality

Categories

Biochemical Research Methods Biochemistry & Molecular Biology

Funding

  1. Academy of Finland [260797, 140964]
  2. ERC Micro-RIP [615146]
  3. Academy of Finland (AKA) [140964, 140964, 260797] Funding Source: Academy of Finland (AKA)
  4. European Research Council (ERC) [615146] Funding Source: European Research Council (ERC)

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Sample barcoding facilitates the analysis of tens or even hundreds of samples in a single next-generation sequencing (NGS) run, but more efficient methods are needed for high-throughput barcoding and size-trimming of long PCR products. Here we present a two-step PCR approach for barcoding followed by pool shearing, adapter ligation, and 5' end selection for trimming sets of DNA templates of any size. Our new trimming method offers clear benefits for phylogenetic studies, since targeting exactly the same region maximizes the alignment and enables the use of operational taxonomic unit (OTU)-based algorithms.

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