Copy Number Variation in Inflammatory Breast Cancer

Aditi Hazra; Andrea O'Hara; Kornelia Polyak; Faina Nakhlis; Beth T Harrison; Antonio Giordano; Beth Overmoyer; Filipa Lynce

doi:10.3390/cells12071086

Copy Number Variation in Inflammatory Breast Cancer

Cells. 2023 Apr 4;12(7):1086. doi: 10.3390/cells12071086.

Authors

Aditi Hazra^{1

2}, Andrea O'Hara³, Kornelia Polyak^{2

4}, Faina Nakhlis^{2

5}, Beth T Harrison^{2

6}, Antonio Giordano^{2

4}, Beth Overmoyer^{2

4}, Filipa Lynce^{2

4}

Affiliations

¹ Division of Preventive Medicine, Brigham and Women's Hospital, Harvard Medical School, Boston, MA 02215, USA.
² Inflammatory Breast Cancer Program, Dana-Farber Cancer Institute, Boston, MA 02115, USA.
³ Bionano Genomics, San Diego, CA 92121, USA.
⁴ Department of Medical Oncology, Breast Oncology Center, Dana-Farber Cancer Institute, Harvard Medical School, Boston, MA 02115, USA.
⁵ Department of Surgery, Division of Breast Surgery, Brigham and Women's Hospital, Harvard Medical School, Boston, MA 02115, USA.
⁶ Department of Pathology, Brigham and Women's Hospital, Harvard Medical School, Boston, MA 02115, USA.

Abstract

Identification of a unique genomic biomarker in de novo inflammatory breast cancer (IBC) may provide an insight into the biology of this aggressive disease. The goal of our study was to elucidate biomarkers associated with IBC. We examined breast biopsies collected from Dana-Farber Cancer Institute patients with IBC prior to initiating preoperative systemic treatment (30 samples were examined, of which 14 were eligible). Patients without available biopsies (n = 1), with insufficient tumor epithelial cells (n = 10), or insufficient DNA yield (n = 5) were excluded from the analysis. Molecular subtype and tumor grade were abstracted from a medical records' review. Ten IBC tumors were estrogen-receptor-positive (ER+) and human epidermal growth factor receptor 2 (HER2)-negative (n = 10 out of 14). Sufficient RNA and DNA were simultaneously extracted from 14 biopsy specimens using the Qiagen AllPrep Kit. RNA was amplified using the Sensation kit and profiled using the Affymetrix Human Transcriptome Array 2.0. DNA was profiled for genome-wide copy number variation (CNV) using the Affymetrix OncoScan Array and analyzed using the Nexus Chromosome Analysis Suite. Among the 14 eligible samples, we first confirmed biological concordance and quality control metrics using replicates and gene expression data. Second, we examined CNVs and gene expression change by IBC subtype. We identified significant CNVs in IBC patients after adjusting for multiple comparisons. Next, to assess whether the CNVs were unique to IBC, we compared the IBC CNV data to fresh-frozen non-IBC CNV data from The Cancer Genome Atlas (n = 388). On chromosome 7p11.2, we identified significant CN gain located at position 58,019,983-58,025,423 in 8 ER+ IBC samples compared to 338 non-IBC ER+ samples (region length: 5440 bp gain and 69,039 bp, False Discovery Rate (FDR) p-value = 3.12 × 10^-10) and at position 57,950,944-58,025,423 in 3 TN-IBC samples compared to 50 non-IBC TN samples (74,479 base pair, gain, FDR p-value = 4.27 × 10^-5; near the EGFR gene). We also observed significant CN loss on chromosome 21, located at position 9,648,315-9,764,385 (p-value = 4.27 × 10^-5). Secondarily, differential gene expression in IBC patients with 7p11.2 CN gain compared to SUM149 were explored after FDR correction for multiple testing (p-value = 0.0016), but the results should be interpreted with caution due to the small sample size. Finally, the data presented are hypothesis-generating. Validation of CNVs that contribute to the unique presentation and biological features associated with IBC in larger datasets may lead to the optimization of treatment strategies.

Keywords: EGFR; chromosome 7p11; copy number alterations; copy number variation; inflammatory breast cancer; multi-omics; subtype; triple-negative.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Biomarkers, Tumor
Breast / metabolism
DNA Copy Number Variations / genetics
Humans
Inflammatory Breast Neoplasms* / genetics
Inflammatory Breast Neoplasms* / pathology
RNA

Substances

Biomarkers, Tumor
RNA

Grants and funding

This research was supported by the Dana–Farber Cancer Institute Inflammatory Breast Cancer Research Fund and the Reardon Family Fund (Lynce). The Affymetrix Tumor Profiling—North America Grant (Hazra) provided the OncoScan Gene Chip and Human Transcriptome Array and reagents for nucleic acid extraction and profiling of IBC patient specimens. HTA analysis Expression Console and TAC software were provided by Affymetrix (Travis Burleson) and Thermo Fisher. ChAS software and Nexus software for copy number analyses were provided by Biodiscovery/Bionano Genomics. The American Cancer Society 130793-RSG-17-016-01-CPHPS supported data analyses.