Analyzing and minimizing PCR amplification bias in Illumina sequencing libraries

Aird, Daniel; Ross, Michael G.; Chen, Weisheng; Danielsson, Maxwell; Fennell, Timothy; Russ, Carsten; Jaffe, David B.; Nusbaum, Chad; Gnirke, Andreas

doi:10.1186/gb-2011-12-2-r18

Cited by 1,002 publications

(914 citation statements)

References 22 publications

(28 reference statements)

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“…The level 2 metric is a measure of which exons failed to achieve 50Â unique coverage at 95% of exonic positions; this is frequently the first exon of genes, which are often GCrich and therefore difficult to amplify by PCR and/or to capture by fluid-phase targeted hybrid capture. 51 Of the 14 exons that failed this level of QC on an average validation run, 2 exons are entirely noncoding; according to the COS-MIC database, no recurrent mutations are reported in the remaining 12 exons. It is unlikely, therefore, that a clinically important mutation would be missed because of the lower coverage in these regions.…”

Section: Discussionmentioning

confidence: 99%

Validation of a Next-Generation Sequencing Assay for Clinical Molecular Oncology

Cottrell

Al-Kateb

Bredemeyer

et al. 2014

The Journal of Molecular Diagnostics

169

133

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Currently, oncology testing includes molecular studies and cytogenetic analysis to detect genetic aberrations of clinical significance. Next-generation sequencing (NGS) allows rapid analysis of multiple genes for clinically actionable somatic variants. The WUCaMP assay uses targeted capture for NGS analysis of 25 cancerassociated genes to detect mutations at actionable loci. We present clinical validation of the assay and a detailed framework for design and validation of similar clinical assays. Deep sequencing of 78 tumor specimens (!1000Â average unique coverage across the capture region) achieved high sensitivity for detecting somatic variants at low allele fraction (AF). Validation revealed sensitivities and specificities of 100% for detection of single-nucleotide variants (SNVs) within coding regions, compared with SNP array sequence data (95% CI Z 83.4e100.0 for sensitivity and 94.2e100.0 for specificity) or whole-genome sequencing (95% CI Z 89.1e100.0 for sensitivity and 99.9e100.0 for specificity) of HapMap samples. Sensitivity for detecting variants at an observed 10% AF was 100% (95% CI Z 93.2e100.0) in HapMap mixes. Analysis of 15 masked specimens harboring clinically reported variants yielded concordant calls for 13/13 variants at AF of !15%. The WUCaMP assay is a robust and sensitive method to detect somatic variants of clinical significance in molecular oncology laboratories, with reduced time and cost of genetic analysis allowing for strategic patient management. (J Mol Diagn 2014, 16: 89e105; http://dx.doi.org/10.1016/j.jmoldx.2013 Traditional approaches to the genetic characterization of clinical oncology specimens include cytogenetic analysis, fluorescence in situ hybridization (FISH), and molecular studies of single genes. These methodologies are complementary to each other and generate information of diagnostic and prognostic relevance. However, as new insight is gained into the complexities of cancer at the molecular level, the need emerges to obtain a more detailed cancer genetic profile for improved patient management. As illustrated by recent studies, identifying DNA mutations in cancer may aid in understanding clonal evolution, 1 risk stratification, 2 and therapeutic strategies. 3,4 With the advent of next-generation sequencing (NGS), a more complete biological characterization of a tumor can be attained at the molecular level. 5

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Section: Discussionmentioning

confidence: 99%

Validation of a Next-Generation Sequencing Assay for Clinical Molecular Oncology

Cottrell

Al-Kateb

Bredemeyer

et al. 2014

The Journal of Molecular Diagnostics

169

133

View full text Add to dashboard Cite

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“…Recently it has shown that amplification-free protocols can reduce the bias [which type of bias?] originated from PCR amplification 32,33 . Sequencing coverage of the transcriptome from these protocols is more even and contiguous across transcripts, making it easier to construct full-length transcripts.…”

Section: Library Constructionmentioning

confidence: 99%

Next-generation transcriptome assembly

2011

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“…88 Other than affecting fragmentation, GC content has a relevant impact on cDNA amplification efficiency. 91 GC-rich RNA fragments undergo base pairing and often form double-strand or highly-paired secondary structures that affect -or impede -reverse transcription of such fragments, leading to a dramatic unbalance in PCR products. 90 Furthermore, RNA-to-cDNA conversion (retrotranscription) before sequencing may introduce biases and artifacts interfering with the characterization and quantification of transcripts.…”

Section: Rna-seq In Human Complex Diseasesmentioning

confidence: 99%

“…Other effects, such as the choice of PCR enzyme or instruments have been also raised, and RNA-Seq in human complex diseases V Costa et al globally the PCR amplification has been identified as the most discriminatory step with some relevant hidden factors still to be examined. 91 To overcome the previously cited limitations of RT and amplification, direct single molecule RNA sequencing approach has been developed, 92 in which PCR amplification is no more required. However, the higher error rate compared with other reversible terminator chemistries is a severe issue even for this technology (discussed in Metzker et al 93 ).…”

Section: Rna-seq In Human Complex Diseasesmentioning

confidence: 99%

RNA-Seq and human complex diseases: recent accomplishments and future perspectives

et al. 2012

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Analyzing and minimizing PCR amplification bias in Illumina sequencing libraries

Cited by 1,002 publications

References 22 publications

Validation of a Next-Generation Sequencing Assay for Clinical Molecular Oncology

Validation of a Next-Generation Sequencing Assay for Clinical Molecular Oncology

Next-generation transcriptome assembly

RNA-Seq and human complex diseases: recent accomplishments and future perspectives

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