Formalin fixation increases deamination mutation signature but should not lead to false positive mutations in clinical practice

Genomic analysis of cancer tissues is an essential aspect of personalized oncology treatment. Though it has been suggested that formalin fixation of patient tissues may be suboptimal for molecular studies, this tissue processing approach remains the industry standard. Therefore clinical molecular la...

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Autores principales: Prentice, Leah M., Miller, Ruth R., Knaggs, Jeff, Mazloomian, Alborz, Aguirre Hernandez, Rosalia, Franchini, Patrick, Parsa, Kourosh, Tessier-Cloutier, Basile, Lapuk, Anna, Huntsman, David, Schaeffer, David F., Sheffield, Brandon S.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2018
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Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5919577/
https://www.ncbi.nlm.nih.gov/pubmed/29698444
http://dx.doi.org/10.1371/journal.pone.0196434
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author Prentice, Leah M.
Miller, Ruth R.
Knaggs, Jeff
Mazloomian, Alborz
Aguirre Hernandez, Rosalia
Franchini, Patrick
Parsa, Kourosh
Tessier-Cloutier, Basile
Lapuk, Anna
Huntsman, David
Schaeffer, David F.
Sheffield, Brandon S.
author_facet Prentice, Leah M.
Miller, Ruth R.
Knaggs, Jeff
Mazloomian, Alborz
Aguirre Hernandez, Rosalia
Franchini, Patrick
Parsa, Kourosh
Tessier-Cloutier, Basile
Lapuk, Anna
Huntsman, David
Schaeffer, David F.
Sheffield, Brandon S.
author_sort Prentice, Leah M.
collection PubMed
description Genomic analysis of cancer tissues is an essential aspect of personalized oncology treatment. Though it has been suggested that formalin fixation of patient tissues may be suboptimal for molecular studies, this tissue processing approach remains the industry standard. Therefore clinical molecular laboratories must be able to work with formalin fixed, paraffin embedded (FFPE) material. This study examines the effects of pre-analytic variables introduced by routine pathology processing on specimens used for clinical reports produced by next-generation sequencing technology. Tissue resected from three colorectal cancer patients was subjected to 2, 15, 24, and 48 hour fixation times in neutral buffered formalin. DNA was extracted from all tissues twice, once with uracil-N-glycosylase (UNG) treatment to counter deamination effects, and once without. Of note, deamination events at methylated cytosine, as found at CpG sites, remains unaffected by UNG. After extraction a two-step PCR targeted sequencing method was performed using the Illumina MiSeq and the data was analyzed via a custom-built bioinformatics pipeline, including filtration of reads with mapping quality <30. A larger baseline group of samples (n = 20) was examined to establish if there was a sample performance difference between the two DNA extraction methods, with/without UNG treatment. There was no statistical difference between sequencing performance of the two extraction methods when comparing read counts (raw, mapped, and filtered) and read quality (% mapped, % filtered). Analyzing mutation type, there was no significant difference between mutation calls until the 48 hour fixation treatment. At 48 hours there is a significant increase in C/G->T/A mutations that is not represented in DNA treated with UNG. This suggests these errors may be due to deamination events triggered by a longer fixation time. However the allelic frequency of these events remained below the limit of detection for reportable mutations in this assay (<2%). We do however recommend that suspected intratumoral heterogeneity events be verified by re-sequencing the same FFPE block.
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spelling pubmed-59195772018-05-11 Formalin fixation increases deamination mutation signature but should not lead to false positive mutations in clinical practice Prentice, Leah M. Miller, Ruth R. Knaggs, Jeff Mazloomian, Alborz Aguirre Hernandez, Rosalia Franchini, Patrick Parsa, Kourosh Tessier-Cloutier, Basile Lapuk, Anna Huntsman, David Schaeffer, David F. Sheffield, Brandon S. PLoS One Research Article Genomic analysis of cancer tissues is an essential aspect of personalized oncology treatment. Though it has been suggested that formalin fixation of patient tissues may be suboptimal for molecular studies, this tissue processing approach remains the industry standard. Therefore clinical molecular laboratories must be able to work with formalin fixed, paraffin embedded (FFPE) material. This study examines the effects of pre-analytic variables introduced by routine pathology processing on specimens used for clinical reports produced by next-generation sequencing technology. Tissue resected from three colorectal cancer patients was subjected to 2, 15, 24, and 48 hour fixation times in neutral buffered formalin. DNA was extracted from all tissues twice, once with uracil-N-glycosylase (UNG) treatment to counter deamination effects, and once without. Of note, deamination events at methylated cytosine, as found at CpG sites, remains unaffected by UNG. After extraction a two-step PCR targeted sequencing method was performed using the Illumina MiSeq and the data was analyzed via a custom-built bioinformatics pipeline, including filtration of reads with mapping quality <30. A larger baseline group of samples (n = 20) was examined to establish if there was a sample performance difference between the two DNA extraction methods, with/without UNG treatment. There was no statistical difference between sequencing performance of the two extraction methods when comparing read counts (raw, mapped, and filtered) and read quality (% mapped, % filtered). Analyzing mutation type, there was no significant difference between mutation calls until the 48 hour fixation treatment. At 48 hours there is a significant increase in C/G->T/A mutations that is not represented in DNA treated with UNG. This suggests these errors may be due to deamination events triggered by a longer fixation time. However the allelic frequency of these events remained below the limit of detection for reportable mutations in this assay (<2%). We do however recommend that suspected intratumoral heterogeneity events be verified by re-sequencing the same FFPE block. Public Library of Science 2018-04-26 /pmc/articles/PMC5919577/ /pubmed/29698444 http://dx.doi.org/10.1371/journal.pone.0196434 Text en © 2018 Prentice et al http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Prentice, Leah M.
Miller, Ruth R.
Knaggs, Jeff
Mazloomian, Alborz
Aguirre Hernandez, Rosalia
Franchini, Patrick
Parsa, Kourosh
Tessier-Cloutier, Basile
Lapuk, Anna
Huntsman, David
Schaeffer, David F.
Sheffield, Brandon S.
Formalin fixation increases deamination mutation signature but should not lead to false positive mutations in clinical practice
title Formalin fixation increases deamination mutation signature but should not lead to false positive mutations in clinical practice
title_full Formalin fixation increases deamination mutation signature but should not lead to false positive mutations in clinical practice
title_fullStr Formalin fixation increases deamination mutation signature but should not lead to false positive mutations in clinical practice
title_full_unstemmed Formalin fixation increases deamination mutation signature but should not lead to false positive mutations in clinical practice
title_short Formalin fixation increases deamination mutation signature but should not lead to false positive mutations in clinical practice
title_sort formalin fixation increases deamination mutation signature but should not lead to false positive mutations in clinical practice
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5919577/
https://www.ncbi.nlm.nih.gov/pubmed/29698444
http://dx.doi.org/10.1371/journal.pone.0196434
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