Molecular Oncology
Volume 4, Issue 2 , Pages 161-168, April 2010

Aberrations of ERBB2 and TOP2A genes in breast cancer

  • Kirsten Vang Nielsen

      Affiliations

    • Dako A/S, Glostrup, Denmark
    • Corresponding Author InformationCorresponding author at: Produktionsvej 42, DK-2600 Glostrup, Denmark. Tel.: +45 4485 9494.
    • ,
  • Sven Müller

      Affiliations

    • Dako A/S, Glostrup, Denmark
    • ,
  • Susanne Møller

      Affiliations

    • Danish Breast Cancer Cooperative Group (DBCG) Registry, Copenhagen, Denmark
    • ,
  • Andreas Schønau

      Affiliations

    • Dako A/S, Glostrup, Denmark
    • ,
  • Eva Balslev

      Affiliations

    • Department of Pathology, Herlev University Hospital, Herlev, Denmark
    • ,
  • Ann S. Knoop

      Affiliations

    • Department of Oncology, Odense University Hospital, Odense, Denmark
    • ,
  • Bent Ejlertsen

      Affiliations

    • Danish Breast Cancer Cooperative Group (DBCG) Registry, Copenhagen, Denmark
    • Department of Oncology, Rigshospitalet, Copenhagen University Hospital, Copenhagen, Denmark

Received 2 September 2009; received in revised form 10 November 2009; accepted 11 November 2009. published online 26 November 2009.

Abstract 

Copy number changes in TOP2A have frequently been linked to ERBB2 (HER2) amplified breast cancers. To study this relationship, copy number changes of ERBB2 and TOP2A were investigated by fluorescence in situ hybridization (FISH) in two cell lines; one characterized by having amplification of both genes and the other by having amplification of ERBB2 and deletion of TOP2A. The characteristics are compared to findings on paired ERBB2 and TOP2A data from 649 patients with invasive breast cancer from a previously published biomarker study. The physical localization of FISH signals in metaphase spreads from cell lines showed that simultaneous amplification is not a simple co-amplification of a whole amplicon containing both genes. Most gene signals are translocated to abnormal marker chromosomes. ERBB2 genes but not TOP2A genes are present in tandem amplicons, leading to a higher ERBB2 ratio. This observation was confirmed by patient FISH data: among 276 (43% of all patients) abnormal tumors, 67% had different ERBB2 and TOP2A status. ERBB2 amplification with normal TOP2A status was found in 36% of the abnormal tumors (15% of all patients). Simultaneous amplification of both genes was found in 28% of the abnormal tumors (12% of all patients) while TOP2A deletion and ERBB2 amplification was observed in 16% of the abnormal cases (8% of all patients). A small number of tumors had TOP2A amplification (4%) or deletion (6%) without simultaneous changes of the ERBB2 gene. ERBB2 deletion was also observed (5%) but only in tumors with simultaneous TOP2A deletion. The average gene/reference ratio was significantly different: 5.0 for TOP2A but 7.2 for ERBB2 in the amplified tumors (P<0.01). Amplification of the two genes may be caused by different mechanisms, leading to higher level of amplification for ERBB2 compared to TOP2A. In the majority of breast cancer patients, simultaneous aberration of ERBB2 and TOP2A is not explained by simple co-amplification.

Keywords: TOP2A, ERBB2, HER2, Gene amplification, Gene deletion, Copy number changes, Chromosome aberrations, Breast cancer

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PII: S1574-7891(09)00138-0

doi:10.1016/j.molonc.2009.11.001

Molecular Oncology
Volume 4, Issue 2 , Pages 161-168, April 2010

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