DNA qualification workflow for next generation sequencing of histopathological samples.

DNA qualification workflow for next generation sequencing of histopathological samples.

Histopathological samples are a treasure-trove of DNA for clinical research. However, the quality of DNA can vary depending on the source or extraction method applied. Thus a standardized and cost-effective workflow for the qualification of DNA preparations is essential to guarantee interlaboratory...

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Main Authors: Michele Simbolo, Marisa Gottardi, Vincenzo Corbo, Matteo Fassan, Andrea Mafficini, Giorgio Malpeli, Rita T Lawlor, Aldo Scarpa
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2013-01-01
Series:PLoS ONE
Online Access:https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/23762227/?tool=EBI
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spelling doaj-4092ff80f7aa4b97aba50372a059d4b22021-03-03T23:17:08ZengPublic Library of Science (PLoS)PLoS ONE1932-62032013-01-0186e6269210.1371/journal.pone.0062692DNA qualification workflow for next generation sequencing of histopathological samples.Michele SimboloMarisa GottardiVincenzo CorboMatteo FassanAndrea MafficiniGiorgio MalpeliRita T LawlorAldo ScarpaHistopathological samples are a treasure-trove of DNA for clinical research. However, the quality of DNA can vary depending on the source or extraction method applied. Thus a standardized and cost-effective workflow for the qualification of DNA preparations is essential to guarantee interlaboratory reproducible results. The qualification process consists of the quantification of double strand DNA (dsDNA) and the assessment of its suitability for downstream applications, such as high-throughput next-generation sequencing. We tested the two most frequently used instrumentations to define their role in this process: NanoDrop, based on UV spectroscopy, and Qubit 2.0, which uses fluorochromes specifically binding dsDNA. Quantitative PCR (qPCR) was used as the reference technique as it simultaneously assesses DNA concentration and suitability for PCR amplification. We used 17 genomic DNAs from 6 fresh-frozen (FF) tissues, 6 formalin-fixed paraffin-embedded (FFPE) tissues, 3 cell lines, and 2 commercial preparations. Intra- and inter-operator variability was negligible, and intra-methodology variability was minimal, while consistent inter-methodology divergences were observed. In fact, NanoDrop measured DNA concentrations higher than Qubit and its consistency with dsDNA quantification by qPCR was limited to high molecular weight DNA from FF samples and cell lines, where total DNA and dsDNA quantity virtually coincide. In partially degraded DNA from FFPE samples, only Qubit proved highly reproducible and consistent with qPCR measurements. Multiplex PCR amplifying 191 regions of 46 cancer-related genes was designated the downstream application, using 40 ng dsDNA from FFPE samples calculated by Qubit. All but one sample produced amplicon libraries suitable for next-generation sequencing. NanoDrop UV-spectrum verified contamination of the unsuccessful sample. In conclusion, as qPCR has high costs and is labor intensive, an alternative effective standard workflow for qualification of DNA preparations should include the sequential combination of NanoDrop and Qubit to assess the purity and quantity of dsDNA, respectively.https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/23762227/?tool=EBI
collection DOAJ
language English
format Article
sources DOAJ
author Michele Simbolo
Marisa Gottardi
Vincenzo Corbo
Matteo Fassan
Andrea Mafficini
Giorgio Malpeli
Rita T Lawlor
Aldo Scarpa
spellingShingle Michele Simbolo
Marisa Gottardi
Vincenzo Corbo
Matteo Fassan
Andrea Mafficini
Giorgio Malpeli
Rita T Lawlor
Aldo Scarpa
DNA qualification workflow for next generation sequencing of histopathological samples.
PLoS ONE
author_facet Michele Simbolo
Marisa Gottardi
Vincenzo Corbo
Matteo Fassan
Andrea Mafficini
Giorgio Malpeli
Rita T Lawlor
Aldo Scarpa
author_sort Michele Simbolo
title DNA qualification workflow for next generation sequencing of histopathological samples.
title_short DNA qualification workflow for next generation sequencing of histopathological samples.
title_full DNA qualification workflow for next generation sequencing of histopathological samples.
title_fullStr DNA qualification workflow for next generation sequencing of histopathological samples.
title_full_unstemmed DNA qualification workflow for next generation sequencing of histopathological samples.
title_sort dna qualification workflow for next generation sequencing of histopathological samples.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2013-01-01
description Histopathological samples are a treasure-trove of DNA for clinical research. However, the quality of DNA can vary depending on the source or extraction method applied. Thus a standardized and cost-effective workflow for the qualification of DNA preparations is essential to guarantee interlaboratory reproducible results. The qualification process consists of the quantification of double strand DNA (dsDNA) and the assessment of its suitability for downstream applications, such as high-throughput next-generation sequencing. We tested the two most frequently used instrumentations to define their role in this process: NanoDrop, based on UV spectroscopy, and Qubit 2.0, which uses fluorochromes specifically binding dsDNA. Quantitative PCR (qPCR) was used as the reference technique as it simultaneously assesses DNA concentration and suitability for PCR amplification. We used 17 genomic DNAs from 6 fresh-frozen (FF) tissues, 6 formalin-fixed paraffin-embedded (FFPE) tissues, 3 cell lines, and 2 commercial preparations. Intra- and inter-operator variability was negligible, and intra-methodology variability was minimal, while consistent inter-methodology divergences were observed. In fact, NanoDrop measured DNA concentrations higher than Qubit and its consistency with dsDNA quantification by qPCR was limited to high molecular weight DNA from FF samples and cell lines, where total DNA and dsDNA quantity virtually coincide. In partially degraded DNA from FFPE samples, only Qubit proved highly reproducible and consistent with qPCR measurements. Multiplex PCR amplifying 191 regions of 46 cancer-related genes was designated the downstream application, using 40 ng dsDNA from FFPE samples calculated by Qubit. All but one sample produced amplicon libraries suitable for next-generation sequencing. NanoDrop UV-spectrum verified contamination of the unsuccessful sample. In conclusion, as qPCR has high costs and is labor intensive, an alternative effective standard workflow for qualification of DNA preparations should include the sequential combination of NanoDrop and Qubit to assess the purity and quantity of dsDNA, respectively.
url https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/23762227/?tool=EBI
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