Correlation Between Quantitative HER-2 Protein Expression and Risk for Brain Metastases in HER-2+ Advanced Breast Cancer Patients Receiving Trastuzumab-Containing Therapy

Author:

Duchnowska Renata12,Biernat Wojciech32,Szostakiewicz Barbara32,Sperinde Jeff4,Piette Fanny5,Haddad Mojgan4,Paquet Agnes4,Lie Yolanda4,Czartoryska-Arłukowicz Bogumiła62,Wysocki Piotr72,Jankowski Tomasz8,Radecka Barbara9,Foszczyńska-Kłoda Małgorzata102,Litwiniuk Maria112,Dȩbska Sylwia122,Weidler Jodi4,Huang Weidong4,Buyse Marc5,Bates Michael13,Jassem Jacek132

Affiliation:

1. a Military Institute of Medicine, Warsaw, Poland;

2. m Polish Brain Metastasis Consortium

3. b Medical University of Gdańsk, Gdańsk, Poland;

4. c Monogram Biosciences, South San Francisco, California, USA;

5. d International Drug Development Institute, Louvain-la-Neuve, Belgium;

6. e Białystok Oncology Center, Białystok, Poland;

7. f Great Poland Cancer Center, Poznań, Poland;

8. g Lublin Oncology Center, Lublin, Poland;

9. h Opole Oncology Center, Opole, Poland;

10. i West Pomeranian Oncology Center, Szczecin, Poland;

11. j Poznań University of Medical Sciences, Poznań, Poland;

12. k Regional Cancer Center, eŁódź, Poland

13. l Oncology Research and Development, Cepheid, Sunnyvale, California, USA;

Abstract

Abstract Background. Patients with human epidermal growth factor receptor (HER)-2+ breast cancer are at particularly high risk for brain metastases; however, the biological basis is not fully understood. Using a novel HER-2 assay, we investigated the correlation between quantitative HER-2 expression in primary breast cancers and the time to brain metastasis (TTBM) in HER-2+ advanced breast cancer patients treated with trastuzumab. Methods. The study group included 142 consecutive patients who were administered trastuzumab-based therapy for HER-2+ metastatic breast cancer. HER-2/neu gene copy number was quantified as the HER-2/centromeric probe for chromosome 17 (CEP17) ratio by central laboratory fluorescence in situ hybridization (FISH). HER-2 protein was quantified as total HER-2 protein expression (H2T) by the HERmark® assay (Monogram Biosciences, Inc., South San Francisco, CA) in formalin-fixed, paraffin-embedded tumor samples. HER-2 variables were correlated with clinical features and TTBM was measured from the initiation of trastuzumab-containing therapy. Results. A higher H2T level (continuous variable) was correlated with shorter TTBM, whereas HER-2 amplification by FISH and a continuous HER-2/CEP17 ratio were not predictive (p = .013, .28, and .25, respectively). In the subset of patients that was centrally determined by FISH to be HER-2+, an above-the-median H2T level was significantly associated with a shorter TTBM (hazard ratio, [HR], 2.4; p = .005), whereas this was not true for the median HER-2/CEP17 ratio by FISH (p = .4). Correlation between a continuous H2T level and TTBM was confirmed on multivariate analysis (HR, 3.3; p = .024). Conclusions. These data reveal a strong relationship between the quantitative HER-2 protein expression level and the risk for brain relapse in HER-2+ advanced breast cancer patients. Consequently, quantitative assessment of HER-2 protein expression may inform and facilitate refinements in therapeutic treatment strategies for selected subpopulations of patients in this group.

Publisher

Oxford University Press (OUP)

Subject

Cancer Research,Oncology

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