Establishing community reference samples, data and call sets for benchmarking cancer mutation detection using whole-genome sequencing

The Somatic Mutation Working Group of Sequencing Quality Control Phase II Consortium

doi:10.1038/s41587-021-00993-6

Establishing community reference samples, data and call sets for benchmarking cancer mutation detection using whole-genome sequencing

The Somatic Mutation Working Group of Sequencing Quality Control Phase II Consortium

生命科学学院

Roche Sequencing Solutions
National Institutes of Health
Leidos Inc
Loma Linda University Health
The First Affiliated Hospital of Guangzhou Medical University
American Type Culture Collection
AbbVie
Fudan University
Illumina, Inc.
Novartis
Genentech, Inc
Palacký University Olomouc
EATRIS ERIC
IRCCS Centro di Riferimento Oncologico - Aviano PN
Perron Institute for Neurological and Translational Science
University of Tartu
University of Helsinki
Uppsala University
Virginia Polytechnic Institute and State University
Sentieon Inc.
Immuneering Corporation
United States Food and Drug Administration
10x Genomics
Translational Genomics Research Institute
Cornell University
Pacific Biosciences
University of Toledo
University of Hawai'i at Mānoa
Digicon
Environmental Laboratory
SAS Institute, Inc.
Bristol-Myers Squibb
United States Environmental Protection Agency
Q2 Solutions
Kinghorn Cancer Centre
Office of the Commissioner
National Institute of Metrology China
AstraZeneca Pharmaceuticals LP
University of Southern Mississippi

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79 引用（Scopus）

摘要

The lack of samples for generating standardized DNA datasets for setting up a sequencing pipeline or benchmarking the performance of different algorithms limits the implementation and uptake of cancer genomics. Here, we describe reference call sets obtained from paired tumor–normal genomic DNA (gDNA) samples derived from a breast cancer cell line—which is highly heterogeneous, with an aneuploid genome, and enriched in somatic alterations—and a matched lymphoblastoid cell line. We partially validated both somatic mutations and germline variants in these call sets via whole-exome sequencing (WES) with different sequencing platforms and targeted sequencing with >2,000-fold coverage, spanning 82% of genomic regions with high confidence. Although the gDNA reference samples are not representative of primary cancer cells from a clinical sample, when setting up a sequencing pipeline, they not only minimize potential biases from technologies, assays and informatics but also provide a unique resource for benchmarking ‘tumor-only’ or ‘matched tumor–normal’ analyses.

源语言	英语
页（从-至）	1151-1160
页数	10
期刊	Nature Biotechnology
卷	39
期	9
DOI	https://doi.org/10.1038/s41587-021-00993-6
出版状态	已出版 - 9月 2021

联合国可持续发展目标

此成果有助于实现下列可持续发展目标：

可持续发展目标 3 良好健康与福祉

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10.1038/s41587-021-00993-6

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title = "Establishing community reference samples, data and call sets for benchmarking cancer mutation detection using whole-genome sequencing",

abstract = "The lack of samples for generating standardized DNA datasets for setting up a sequencing pipeline or benchmarking the performance of different algorithms limits the implementation and uptake of cancer genomics. Here, we describe reference call sets obtained from paired tumor–normal genomic DNA (gDNA) samples derived from a breast cancer cell line—which is highly heterogeneous, with an aneuploid genome, and enriched in somatic alterations—and a matched lymphoblastoid cell line. We partially validated both somatic mutations and germline variants in these call sets via whole-exome sequencing (WES) with different sequencing platforms and targeted sequencing with >2,000-fold coverage, spanning 82\% of genomic regions with high confidence. Although the gDNA reference samples are not representative of primary cancer cells from a clinical sample, when setting up a sequencing pipeline, they not only minimize potential biases from technologies, assays and informatics but also provide a unique resource for benchmarking {\textquoteleft}tumor-only{\textquoteright} or {\textquoteleft}matched tumor–normal{\textquoteright} analyses.",

author = "\{The Somatic Mutation Working Group of Sequencing Quality Control Phase II Consortium\} and Fang, \{Li Tai\} and Bin Zhu and Yongmei Zhao and Wanqiu Chen and Zhaowei Yang and Liz Kerrigan and Kurt Langenbach and \{de Mars\}, Maryellen and Charles Lu and Kenneth Idler and Howard Jacob and Yuanting Zheng and Luyao Ren and Ying Yu and Erich Jaeger and Schroth, \{Gary P.\} and Abaan, \{Ogan D.\} and Keyur Talsania and Justin Lack and Shen, \{Tsai Wei\} and Zhong Chen and Seta Stanbouly and Bao Tran and Jyoti Shetty and Yuliya Kriga and Daoud Meerzaman and Cu Nguyen and Virginie Petitjean and Marc Sultan and Margaret Cam and Monika Mehta and Tiffany Hung and Eric Peters and Rasika Kalamegham and Sahraeian, \{Sayed Mohammad Ebrahim\} and Marghoob Mohiyuddin and Yunfei Guo and Lijing Yao and Lei Song and Lam, \{Hugo Y.K.\} and Jiri Drabek and Petr Vojta and Roberta Maestro and Daniela Gasparotto and Sulev K{\"o}ks and Ene Reimann and Andreas Scherer and Jessica Nordlund and Ulrika Liljedahl and Tieliu Shi",

note = "Publisher Copyright: {\textcopyright} 2021, This is a U.S. government work and not under copyright protection in the U.S.; foreign copyright protection may apply.",

year = "2021",

month = sep,

doi = "10.1038/s41587-021-00993-6",

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AU - Zhao, Yongmei

AU - Chen, Wanqiu

AU - Yang, Zhaowei

AU - Kerrigan, Liz

AU - Langenbach, Kurt

AU - de Mars, Maryellen

AU - Lu, Charles

AU - Idler, Kenneth

AU - Jacob, Howard

AU - Zheng, Yuanting

AU - Ren, Luyao

AU - Yu, Ying

AU - Jaeger, Erich

AU - Schroth, Gary P.

AU - Abaan, Ogan D.

AU - Talsania, Keyur

AU - Lack, Justin

AU - Shen, Tsai Wei

AU - Chen, Zhong

AU - Stanbouly, Seta

AU - Tran, Bao

AU - Shetty, Jyoti

AU - Kriga, Yuliya

AU - Meerzaman, Daoud

AU - Nguyen, Cu

AU - Petitjean, Virginie

AU - Sultan, Marc

AU - Cam, Margaret

AU - Mehta, Monika

AU - Hung, Tiffany

AU - Peters, Eric

AU - Kalamegham, Rasika

AU - Sahraeian, Sayed Mohammad Ebrahim

AU - Mohiyuddin, Marghoob

AU - Guo, Yunfei

AU - Yao, Lijing

AU - Song, Lei

AU - Lam, Hugo Y.K.

AU - Drabek, Jiri

AU - Vojta, Petr

AU - Maestro, Roberta

AU - Gasparotto, Daniela

AU - Köks, Sulev

AU - Reimann, Ene

AU - Scherer, Andreas

AU - Nordlund, Jessica

AU - Liljedahl, Ulrika

AU - Shi, Tieliu

PY - 2021/9

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N2 - The lack of samples for generating standardized DNA datasets for setting up a sequencing pipeline or benchmarking the performance of different algorithms limits the implementation and uptake of cancer genomics. Here, we describe reference call sets obtained from paired tumor–normal genomic DNA (gDNA) samples derived from a breast cancer cell line—which is highly heterogeneous, with an aneuploid genome, and enriched in somatic alterations—and a matched lymphoblastoid cell line. We partially validated both somatic mutations and germline variants in these call sets via whole-exome sequencing (WES) with different sequencing platforms and targeted sequencing with >2,000-fold coverage, spanning 82% of genomic regions with high confidence. Although the gDNA reference samples are not representative of primary cancer cells from a clinical sample, when setting up a sequencing pipeline, they not only minimize potential biases from technologies, assays and informatics but also provide a unique resource for benchmarking ‘tumor-only’ or ‘matched tumor–normal’ analyses.

AB - The lack of samples for generating standardized DNA datasets for setting up a sequencing pipeline or benchmarking the performance of different algorithms limits the implementation and uptake of cancer genomics. Here, we describe reference call sets obtained from paired tumor–normal genomic DNA (gDNA) samples derived from a breast cancer cell line—which is highly heterogeneous, with an aneuploid genome, and enriched in somatic alterations—and a matched lymphoblastoid cell line. We partially validated both somatic mutations and germline variants in these call sets via whole-exome sequencing (WES) with different sequencing platforms and targeted sequencing with >2,000-fold coverage, spanning 82% of genomic regions with high confidence. Although the gDNA reference samples are not representative of primary cancer cells from a clinical sample, when setting up a sequencing pipeline, they not only minimize potential biases from technologies, assays and informatics but also provide a unique resource for benchmarking ‘tumor-only’ or ‘matched tumor–normal’ analyses.

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DO - 10.1038/s41587-021-00993-6

M3 - 文章

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AN - SCOPUS:85115970978

SN - 1087-0156

VL - 39

SP - 1151

EP - 1160

JO - Nature Biotechnology

JF - Nature Biotechnology

IS - 9

ER -

Establishing community reference samples, data and call sets for benchmarking cancer mutation detection using whole-genome sequencing

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