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Integrated Analysis of Gene Expression, CpG Island Methylation, and Gene Copy Number in Breast Cancer Cells by Deep Sequencing

Overview of attention for article published in PLOS ONE, February 2011
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Title
Integrated Analysis of Gene Expression, CpG Island Methylation, and Gene Copy Number in Breast Cancer Cells by Deep Sequencing
Published in
PLOS ONE, February 2011
DOI 10.1371/journal.pone.0017490
Pubmed ID
Authors

Zhifu Sun, Yan W. Asmann, Krishna R. Kalari, Brian Bot, Jeanette E. Eckel-Passow, Tiffany R. Baker, Jennifer M. Carr, Irina Khrebtukova, Shujun Luo, Lu Zhang, Gary P. Schroth, Edith A. Perez, E. Aubrey Thompson

Abstract

We used deep sequencing technology to profile the transcriptome, gene copy number, and CpG island methylation status simultaneously in eight commonly used breast cell lines to develop a model for how these genomic features are integrated in estrogen receptor positive (ER+) and negative breast cancer. Total mRNA sequence, gene copy number, and genomic CpG island methylation were carried out using the Illumina Genome Analyzer. Sequences were mapped to the human genome to obtain digitized gene expression data, DNA copy number in reference to the non-tumor cell line (MCF10A), and methylation status of 21,570 CpG islands to identify differentially expressed genes that were correlated with methylation or copy number changes. These were evaluated in a dataset from 129 primary breast tumors. Gene expression in cell lines was dominated by ER-associated genes. ER+ and ER- cell lines formed two distinct, stable clusters, and 1,873 genes were differentially expressed in the two groups. Part of chromosome 8 was deleted in all ER- cells and part of chromosome 17 amplified in all ER+ cells. These loci encoded 30 genes that were overexpressed in ER+ cells; 9 of these genes were overexpressed in ER+ tumors. We identified 149 differentially expressed genes that exhibited differential methylation of one or more CpG islands within 5 kb of the 5' end of the gene and for which mRNA abundance was inversely correlated with CpG island methylation status. In primary tumors we identified 84 genes that appear to be robust components of the methylation signature that we identified in ER+ cell lines. Our analyses reveal a global pattern of differential CpG island methylation that contributes to the transcriptome landscape of ER+ and ER- breast cancer cells and tumors. The role of gene amplification/deletion appears to more modest, although several potentially significant genes appear to be regulated by copy number aberrations.

Mendeley readers

Mendeley readers

The data shown below were compiled from readership statistics for 244 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
United States 8 3%
Germany 3 1%
Netherlands 1 <1%
France 1 <1%
Norway 1 <1%
Italy 1 <1%
Turkey 1 <1%
Sweden 1 <1%
Israel 1 <1%
Other 6 2%
Unknown 220 90%

Demographic breakdown

Readers by professional status Count As %
Researcher 79 32%
Student > Ph. D. Student 55 23%
Professor > Associate Professor 21 9%
Student > Master 18 7%
Other 13 5%
Other 42 17%
Unknown 16 7%
Readers by discipline Count As %
Agricultural and Biological Sciences 118 48%
Biochemistry, Genetics and Molecular Biology 41 17%
Medicine and Dentistry 20 8%
Computer Science 16 7%
Mathematics 6 2%
Other 22 9%
Unknown 21 9%
Attention Score in Context

Attention Score in Context

This research output has an Altmetric Attention Score of 1. This is our high-level measure of the quality and quantity of online attention that it has received. This Attention Score, as well as the ranking and number of research outputs shown below, was calculated when the research output was last mentioned on 19 May 2012.
All research outputs
#20,157,329
of 22,665,794 outputs
Outputs from PLOS ONE
#172,668
of 193,511 outputs
Outputs of similar age
#100,071
of 106,455 outputs
Outputs of similar age from PLOS ONE
#1,254
of 1,332 outputs
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