Quantifying sequencing error and effective sequencing depth of liquid biopsy NGS with UMI error correction

Malene Støchkel Frank; Janina Fuß; Tim Alexander Steiert; Greta Streleckiene; Julie Gehl; Michael Forster

doi:10.2144/btn-2020-0124

Quantifying sequencing error and effective sequencing depth of liquid biopsy NGS with UMI error correction

Malene Støchkel Frank, Janina Fuß, Tim Alexander Steiert, Greta Streleckiene, Julie Gehl, Michael Forster

Publikation: Bidrag til tidsskrift › Tidsskriftartikel › Forskning › peer review

7 Citationer (Scopus)

52 Downloads (Pure)

Abstract

Liquid biopsies are a minimally invasive method to diagnose and longitudinally monitor tumor mutations in patients when tissue biopsies are difficult (e.g., in lung cancer). The percentage of cell-free tumor DNA in blood plasma ranges from more than 65% to 0.1% or lower. To reliably diagnose tumor mutations at 0.1%, there are two options: unrealistically large volumes of patient blood or library preparation and sequencing depth optimized to low-input DNA. Here, we assess two library preparation methods and analysis workflows to determine feasibility and reliability based on standards with known allelic frequency (0 and 0.13% in PIK3CA). However, the implementation for patients is still costly and requires elaborate setups.

Originalsprog	Engelsk
Tidsskrift	BioTechniques
Vol/bind	70
Udgave nummer	4
Sider (fra-til)	226-232
Antal sider	7
ISSN	0736-6205
DOI	https://doi.org/10.2144/btn-2020-0124
Status	Udgivet - 2021

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10.2144/btn-2020-0124Licens: CC BY-NC-ND

Quantifying sequencing error and effective sequencing depth of liquid biopsy NGS with UMI error correctionForlagets udgivne version, 428 KBLicens: CC BY-NC-ND

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abstract = "Liquid biopsies are a minimally invasive method to diagnose and longitudinally monitor tumor mutations in patients when tissue biopsies are difficult (e.g., in lung cancer). The percentage of cell-free tumor DNA in blood plasma ranges from more than 65% to 0.1% or lower. To reliably diagnose tumor mutations at 0.1%, there are two options: unrealistically large volumes of patient blood or library preparation and sequencing depth optimized to low-input DNA. Here, we assess two library preparation methods and analysis workflows to determine feasibility and reliability based on standards with known allelic frequency (0 and 0.13% in PIK3CA). However, the implementation for patients is still costly and requires elaborate setups.",

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T1 - Quantifying sequencing error and effective sequencing depth of liquid biopsy NGS with UMI error correction

AU - Frank, Malene Støchkel

AU - Fuß, Janina

AU - Steiert, Tim Alexander

AU - Streleckiene, Greta

AU - Gehl, Julie

AU - Forster, Michael

PY - 2021

Y1 - 2021

N2 - Liquid biopsies are a minimally invasive method to diagnose and longitudinally monitor tumor mutations in patients when tissue biopsies are difficult (e.g., in lung cancer). The percentage of cell-free tumor DNA in blood plasma ranges from more than 65% to 0.1% or lower. To reliably diagnose tumor mutations at 0.1%, there are two options: unrealistically large volumes of patient blood or library preparation and sequencing depth optimized to low-input DNA. Here, we assess two library preparation methods and analysis workflows to determine feasibility and reliability based on standards with known allelic frequency (0 and 0.13% in PIK3CA). However, the implementation for patients is still costly and requires elaborate setups.

AB - Liquid biopsies are a minimally invasive method to diagnose and longitudinally monitor tumor mutations in patients when tissue biopsies are difficult (e.g., in lung cancer). The percentage of cell-free tumor DNA in blood plasma ranges from more than 65% to 0.1% or lower. To reliably diagnose tumor mutations at 0.1%, there are two options: unrealistically large volumes of patient blood or library preparation and sequencing depth optimized to low-input DNA. Here, we assess two library preparation methods and analysis workflows to determine feasibility and reliability based on standards with known allelic frequency (0 and 0.13% in PIK3CA). However, the implementation for patients is still costly and requires elaborate setups.

KW - cell-free DNA

KW - low allele frequency

KW - next-generation sequencing

KW - unique molecular identifier (UMI)

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JO - BioTechniques

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