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Optical mapping reveals a higher level of genomic architecture of chained fusions in cancer

Genomic rearrangements are common in cancer, with demonstrated links to disease progression and treatment response. These rearrangements can be complex, resulting in fusions of multiple chromosomal fragments and generation of derivative chromosomes. Although methods exist for detecting individual fu...

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Autores principales: Chan, Eva K.F., Cameron, Daniel L., Petersen, Desiree C., Lyons, Ruth J., Baldi, Benedetta F., Papenfuss, Anthony T., Thomas, David M., Hayes, Vanessa M.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Cold Spring Harbor Laboratory Press 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5932612/
https://www.ncbi.nlm.nih.gov/pubmed/29618486
http://dx.doi.org/10.1101/gr.227975.117
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author Chan, Eva K.F.
Cameron, Daniel L.
Petersen, Desiree C.
Lyons, Ruth J.
Baldi, Benedetta F.
Papenfuss, Anthony T.
Thomas, David M.
Hayes, Vanessa M.
author_facet Chan, Eva K.F.
Cameron, Daniel L.
Petersen, Desiree C.
Lyons, Ruth J.
Baldi, Benedetta F.
Papenfuss, Anthony T.
Thomas, David M.
Hayes, Vanessa M.
author_sort Chan, Eva K.F.
collection PubMed
description Genomic rearrangements are common in cancer, with demonstrated links to disease progression and treatment response. These rearrangements can be complex, resulting in fusions of multiple chromosomal fragments and generation of derivative chromosomes. Although methods exist for detecting individual fusions, they are generally unable to reconstruct complex chained events. To overcome these limitations, we adopted a new optical mapping approach, allowing megabase-length genome maps to be reconstructed and rearranged genomes to be visualized without loss of integrity. Whole-genome mapping (Bionano Genomics) of a well-studied highly rearranged liposarcoma cell line resulted in 3338 assembled consensus genome maps, including 72 fusion maps. These fusion maps represent 112.3 Mb of highly rearranged genomic regions, illuminating the complex architecture of chained fusions, including content, order, orientation, and size. Spanning the junction of 147 chromosomal translocations, we found a total of 28 Mb of interspersed sequences that could not be aligned to the reference genome. Traversing these interspersed sequences using short-read sequencing breakpoint calls, we were able to identify and place 399 sequencing fragments within the optical mapping gaps, thus illustrating the complementary nature of optical mapping and short-read sequencing. We demonstrate that optical mapping provides a powerful new approach for capturing a higher level of complex genomic architecture, creating a scaffold for renewed interpretation of sequencing data of particular relevance to human cancer.
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spelling pubmed-59326122018-05-31 Optical mapping reveals a higher level of genomic architecture of chained fusions in cancer Chan, Eva K.F. Cameron, Daniel L. Petersen, Desiree C. Lyons, Ruth J. Baldi, Benedetta F. Papenfuss, Anthony T. Thomas, David M. Hayes, Vanessa M. Genome Res Method Genomic rearrangements are common in cancer, with demonstrated links to disease progression and treatment response. These rearrangements can be complex, resulting in fusions of multiple chromosomal fragments and generation of derivative chromosomes. Although methods exist for detecting individual fusions, they are generally unable to reconstruct complex chained events. To overcome these limitations, we adopted a new optical mapping approach, allowing megabase-length genome maps to be reconstructed and rearranged genomes to be visualized without loss of integrity. Whole-genome mapping (Bionano Genomics) of a well-studied highly rearranged liposarcoma cell line resulted in 3338 assembled consensus genome maps, including 72 fusion maps. These fusion maps represent 112.3 Mb of highly rearranged genomic regions, illuminating the complex architecture of chained fusions, including content, order, orientation, and size. Spanning the junction of 147 chromosomal translocations, we found a total of 28 Mb of interspersed sequences that could not be aligned to the reference genome. Traversing these interspersed sequences using short-read sequencing breakpoint calls, we were able to identify and place 399 sequencing fragments within the optical mapping gaps, thus illustrating the complementary nature of optical mapping and short-read sequencing. We demonstrate that optical mapping provides a powerful new approach for capturing a higher level of complex genomic architecture, creating a scaffold for renewed interpretation of sequencing data of particular relevance to human cancer. Cold Spring Harbor Laboratory Press 2018-05 /pmc/articles/PMC5932612/ /pubmed/29618486 http://dx.doi.org/10.1101/gr.227975.117 Text en © 2018 Chan et al.; Published by Cold Spring Harbor Laboratory Press http://creativecommons.org/licenses/by/4.0/ This article, published in Genome Research, is available under a Creative Commons License (Attribution 4.0 International), as described at http://creativecommons.org/licenses/by/4.0/.
spellingShingle Method
Chan, Eva K.F.
Cameron, Daniel L.
Petersen, Desiree C.
Lyons, Ruth J.
Baldi, Benedetta F.
Papenfuss, Anthony T.
Thomas, David M.
Hayes, Vanessa M.
Optical mapping reveals a higher level of genomic architecture of chained fusions in cancer
title Optical mapping reveals a higher level of genomic architecture of chained fusions in cancer
title_full Optical mapping reveals a higher level of genomic architecture of chained fusions in cancer
title_fullStr Optical mapping reveals a higher level of genomic architecture of chained fusions in cancer
title_full_unstemmed Optical mapping reveals a higher level of genomic architecture of chained fusions in cancer
title_short Optical mapping reveals a higher level of genomic architecture of chained fusions in cancer
title_sort optical mapping reveals a higher level of genomic architecture of chained fusions in cancer
topic Method
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5932612/
https://www.ncbi.nlm.nih.gov/pubmed/29618486
http://dx.doi.org/10.1101/gr.227975.117
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