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DNA methylation analysis by digital bisulfite genomic sequencing and digital MethyLight

Alterations in cytosine-5 DNA methylation are frequently observed in most types of human cancer. Although assays utilizing PCR amplification of bisulfite-converted DNA are widely employed to analyze these DNA methylation alterations, they are generally limited in throughput capacity, detection sensi...

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Autores principales: Weisenberger, Daniel J., Trinh, Binh N., Campan, Mihaela, Sharma, Shikhar, Long, Tiffany I., Ananthnarayan, Suchitra, Liang, Gangning, Esteva, Francisco J., Hortobagyi, Gabriel N., McCormick, Frank, Jones, Peter A., Laird, Peter W.
Formato: Texto
Lenguaje:English
Publicado: Oxford University Press 2008
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2504308/
https://www.ncbi.nlm.nih.gov/pubmed/18628296
http://dx.doi.org/10.1093/nar/gkn455
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author Weisenberger, Daniel J.
Trinh, Binh N.
Campan, Mihaela
Sharma, Shikhar
Long, Tiffany I.
Ananthnarayan, Suchitra
Liang, Gangning
Esteva, Francisco J.
Hortobagyi, Gabriel N.
McCormick, Frank
Jones, Peter A.
Laird, Peter W.
author_facet Weisenberger, Daniel J.
Trinh, Binh N.
Campan, Mihaela
Sharma, Shikhar
Long, Tiffany I.
Ananthnarayan, Suchitra
Liang, Gangning
Esteva, Francisco J.
Hortobagyi, Gabriel N.
McCormick, Frank
Jones, Peter A.
Laird, Peter W.
author_sort Weisenberger, Daniel J.
collection PubMed
description Alterations in cytosine-5 DNA methylation are frequently observed in most types of human cancer. Although assays utilizing PCR amplification of bisulfite-converted DNA are widely employed to analyze these DNA methylation alterations, they are generally limited in throughput capacity, detection sensitivity, and or resolution. Digital PCR, in which a DNA sample is analyzed in distributive fashion over multiple reaction chambers, allows for enumeration of discrete template DNA molecules, as well as sequestration of non-specific primer annealing templates into negative chambers, thereby increasing the signal-to-noise ratio in positive chambers. Here, we have applied digital PCR technology to bisulfite-converted DNA for single-molecule high-resolution DNA methylation analysis and for increased sensitivity DNA methylation detection. We developed digital bisulfite genomic DNA sequencing to efficiently determine single-basepair DNA methylation patterns on single-molecule DNA templates without an interim cloning step. We also developed digital MethyLight, which surpasses traditional MethyLight in detection sensitivity and quantitative accuracy for low quantities of DNA. Using digital MethyLight, we identified single-molecule, cancer-specific DNA hypermethylation events in the CpG islands of RUNX3, CLDN5 and FOXE1 present in plasma samples from breast cancer patients.
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spelling pubmed-25043082008-08-08 DNA methylation analysis by digital bisulfite genomic sequencing and digital MethyLight Weisenberger, Daniel J. Trinh, Binh N. Campan, Mihaela Sharma, Shikhar Long, Tiffany I. Ananthnarayan, Suchitra Liang, Gangning Esteva, Francisco J. Hortobagyi, Gabriel N. McCormick, Frank Jones, Peter A. Laird, Peter W. Nucleic Acids Res Molecular Biology Alterations in cytosine-5 DNA methylation are frequently observed in most types of human cancer. Although assays utilizing PCR amplification of bisulfite-converted DNA are widely employed to analyze these DNA methylation alterations, they are generally limited in throughput capacity, detection sensitivity, and or resolution. Digital PCR, in which a DNA sample is analyzed in distributive fashion over multiple reaction chambers, allows for enumeration of discrete template DNA molecules, as well as sequestration of non-specific primer annealing templates into negative chambers, thereby increasing the signal-to-noise ratio in positive chambers. Here, we have applied digital PCR technology to bisulfite-converted DNA for single-molecule high-resolution DNA methylation analysis and for increased sensitivity DNA methylation detection. We developed digital bisulfite genomic DNA sequencing to efficiently determine single-basepair DNA methylation patterns on single-molecule DNA templates without an interim cloning step. We also developed digital MethyLight, which surpasses traditional MethyLight in detection sensitivity and quantitative accuracy for low quantities of DNA. Using digital MethyLight, we identified single-molecule, cancer-specific DNA hypermethylation events in the CpG islands of RUNX3, CLDN5 and FOXE1 present in plasma samples from breast cancer patients. Oxford University Press 2008-08 2008-07-15 /pmc/articles/PMC2504308/ /pubmed/18628296 http://dx.doi.org/10.1093/nar/gkn455 Text en © 2008 The Author(s) http://creativecommons.org/licenses/by-nc/2.0/uk/ This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/2.0/uk/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Molecular Biology
Weisenberger, Daniel J.
Trinh, Binh N.
Campan, Mihaela
Sharma, Shikhar
Long, Tiffany I.
Ananthnarayan, Suchitra
Liang, Gangning
Esteva, Francisco J.
Hortobagyi, Gabriel N.
McCormick, Frank
Jones, Peter A.
Laird, Peter W.
DNA methylation analysis by digital bisulfite genomic sequencing and digital MethyLight
title DNA methylation analysis by digital bisulfite genomic sequencing and digital MethyLight
title_full DNA methylation analysis by digital bisulfite genomic sequencing and digital MethyLight
title_fullStr DNA methylation analysis by digital bisulfite genomic sequencing and digital MethyLight
title_full_unstemmed DNA methylation analysis by digital bisulfite genomic sequencing and digital MethyLight
title_short DNA methylation analysis by digital bisulfite genomic sequencing and digital MethyLight
title_sort dna methylation analysis by digital bisulfite genomic sequencing and digital methylight
topic Molecular Biology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2504308/
https://www.ncbi.nlm.nih.gov/pubmed/18628296
http://dx.doi.org/10.1093/nar/gkn455
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