Deep sequencing of target linkage assay-identified regions in familial breast cancer: Methods, analysis pipeline and troubleshooting

Juan Manuel Rosa-Rosa; Francisco Javier Gracia-Aznárez; Emily Hodges; Guillermo Pita; Michelle Rooks; Zhenyu Xuan; Arindam Bhattacharjee; Leonardo Brizuela; José M. Silva; Gregory J. Hannon; Javier Benitez

doi:10.1371/journal.pone.0009976

Deep sequencing of target linkage assay-identified regions in familial breast cancer: Methods, analysis pipeline and troubleshooting

Juan Manuel Rosa-Rosa, Francisco Javier Gracia-Aznárez, Emily Hodges, Guillermo Pita, Michelle Rooks, Zhenyu Xuan, Arindam Bhattacharjee, Leonardo Brizuela, José M. Silva, Gregory J. Hannon, Javier Benitez

Research output: Contribution to journal › Article › peer-review

7 Scopus citations

Abstract

Background: The classical candidate-gene approach has failed to identify novel breast cancer susceptibility genes. Nowadays, massive parallel sequencing technology allows the development of studies unaffordable a few years ago. However, analysis protocols are not yet sufficiently developed to extract all information from the huge amount of data obtained. Methodology/Principal Findings: In this study, we performed high throughput sequencing in two regions located on chromosomes 3 and 6, recently identified by linkage studies by our group as candidate regions for harbouring breast cancer susceptibility genes. In order to enrich for the coding regions of all described genes located in both candidate regions, a hybrid-selection method on tiling microarrays was performed. Conclusions/Significance: We developed an analysis pipeline based on SOAP aligner to identify candidate variants with a high real positive confirmation rate (0.89), with which we identified eight variants considered candidates for functional studies. The results suggest that the present strategy might be a valid second step for identifying high penetrance genes

Original language	English
Article number	e9976
Journal	PLoS ONE
Volume	5
Issue number	4
DOIs	https://doi.org/10.1371/journal.pone.0009976
State	Published - 2010
Externally published	Yes

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Rosa-Rosa, J. M., Gracia-Aznárez, F. J., Hodges, E., Pita, G., Rooks, M., Xuan, Z., Bhattacharjee, A., Brizuela, L., Silva, J. M., Hannon, G. J., & Benitez, J. (2010). Deep sequencing of target linkage assay-identified regions in familial breast cancer: Methods, analysis pipeline and troubleshooting. PLoS ONE, 5(4), Article e9976. https://doi.org/10.1371/journal.pone.0009976

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title = "Deep sequencing of target linkage assay-identified regions in familial breast cancer: Methods, analysis pipeline and troubleshooting",

abstract = "Background: The classical candidate-gene approach has failed to identify novel breast cancer susceptibility genes. Nowadays, massive parallel sequencing technology allows the development of studies unaffordable a few years ago. However, analysis protocols are not yet sufficiently developed to extract all information from the huge amount of data obtained. Methodology/Principal Findings: In this study, we performed high throughput sequencing in two regions located on chromosomes 3 and 6, recently identified by linkage studies by our group as candidate regions for harbouring breast cancer susceptibility genes. In order to enrich for the coding regions of all described genes located in both candidate regions, a hybrid-selection method on tiling microarrays was performed. Conclusions/Significance: We developed an analysis pipeline based on SOAP aligner to identify candidate variants with a high real positive confirmation rate (0.89), with which we identified eight variants considered candidates for functional studies. The results suggest that the present strategy might be a valid second step for identifying high penetrance genes",

author = "Rosa-Rosa, {Juan Manuel} and Gracia-Azn{\'a}rez, {Francisco Javier} and Emily Hodges and Guillermo Pita and Michelle Rooks and Zhenyu Xuan and Arindam Bhattacharjee and Leonardo Brizuela and Silva, {Jos{\'e} M.} and Hannon, {Gregory J.} and Javier Benitez",

year = "2010",

doi = "10.1371/journal.pone.0009976",

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T1 - Deep sequencing of target linkage assay-identified regions in familial breast cancer

T2 - Methods, analysis pipeline and troubleshooting

AU - Rosa-Rosa, Juan Manuel

AU - Gracia-Aznárez, Francisco Javier

AU - Hodges, Emily

AU - Pita, Guillermo

AU - Rooks, Michelle

AU - Xuan, Zhenyu

AU - Bhattacharjee, Arindam

AU - Brizuela, Leonardo

AU - Silva, José M.

AU - Hannon, Gregory J.

AU - Benitez, Javier

PY - 2010

Y1 - 2010

N2 - Background: The classical candidate-gene approach has failed to identify novel breast cancer susceptibility genes. Nowadays, massive parallel sequencing technology allows the development of studies unaffordable a few years ago. However, analysis protocols are not yet sufficiently developed to extract all information from the huge amount of data obtained. Methodology/Principal Findings: In this study, we performed high throughput sequencing in two regions located on chromosomes 3 and 6, recently identified by linkage studies by our group as candidate regions for harbouring breast cancer susceptibility genes. In order to enrich for the coding regions of all described genes located in both candidate regions, a hybrid-selection method on tiling microarrays was performed. Conclusions/Significance: We developed an analysis pipeline based on SOAP aligner to identify candidate variants with a high real positive confirmation rate (0.89), with which we identified eight variants considered candidates for functional studies. The results suggest that the present strategy might be a valid second step for identifying high penetrance genes

AB - Background: The classical candidate-gene approach has failed to identify novel breast cancer susceptibility genes. Nowadays, massive parallel sequencing technology allows the development of studies unaffordable a few years ago. However, analysis protocols are not yet sufficiently developed to extract all information from the huge amount of data obtained. Methodology/Principal Findings: In this study, we performed high throughput sequencing in two regions located on chromosomes 3 and 6, recently identified by linkage studies by our group as candidate regions for harbouring breast cancer susceptibility genes. In order to enrich for the coding regions of all described genes located in both candidate regions, a hybrid-selection method on tiling microarrays was performed. Conclusions/Significance: We developed an analysis pipeline based on SOAP aligner to identify candidate variants with a high real positive confirmation rate (0.89), with which we identified eight variants considered candidates for functional studies. The results suggest that the present strategy might be a valid second step for identifying high penetrance genes

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Deep sequencing of target linkage assay-identified regions in familial breast cancer: Methods, analysis pipeline and troubleshooting

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