Soluble EpCAM levels in ascites correlate with positive cytology and neutralize catumaxomab activity in vitro

Andreas Seeber; Agnieszka Martowicz; Gilbert Spizzo; Thomas Buratti; Peter Obrist; Dominic Fong; Guenther Gastl; Gerold Untergasser

doi:10.1186/s12885-015-1371-1

Soluble EpCAM levels in ascites correlate with positive cytology and neutralize catumaxomab activity in vitro

BMC Cancer. 2015 May 7:15:372. doi: 10.1186/s12885-015-1371-1.

Authors

Andreas Seeber^{1

2

3}, Agnieszka Martowicz^{4

5}, Gilbert Spizzo^{6

7

8}, Thomas Buratti⁹, Peter Obrist¹⁰, Dominic Fong^{11

12}, Guenther Gastl¹³, Gerold Untergasser^{14

15

16}

Affiliations

¹ Experimental Oncogenomics, Tyrolean Cancer Research Institute, Innsbruck, Austria. andreas.seeber@uki.at.
² Oncotyrol - Center for Personalized Cancer Medicine, Innsbruck, Austria. andreas.seeber@uki.at.
³ Department of Hematology and Oncology, Medical University of Innsbruck, Innsbruck, Austria. andreas.seeber@uki.at.
⁴ Experimental Oncogenomics, Tyrolean Cancer Research Institute, Innsbruck, Austria. agnieszka.martowicz@ki.se.
⁵ Division of Vascular Biology, Department of Medical Biochemistry and Biophysics, Karolinska Institute, Stockholm, Sweden. agnieszka.martowicz@ki.se.
⁶ Experimental Oncogenomics, Tyrolean Cancer Research Institute, Innsbruck, Austria. gilbert.spizzo@i-med.ac.at.
⁷ Oncotyrol - Center for Personalized Cancer Medicine, Innsbruck, Austria. gilbert.spizzo@i-med.ac.at.
⁸ Hemato-Oncological Day Hospital, Hospital of Merano, Merano, Italy. gilbert.spizzo@i-med.ac.at.
⁹ Department of Internal Medicine, Hospital of Merano, Merano, Italy. thomas.buratti@asbmeran-o.it.
¹⁰ Pathology Laboratory, Hospital of Zams, Zams, Austria. peter.obrist@tyrolpath.at.
¹¹ Experimental Oncogenomics, Tyrolean Cancer Research Institute, Innsbruck, Austria. dominic.fong@i-med.ac.at.
¹² Hemato-Oncological Day Hospital, Hospital of Merano, Merano, Italy. dominic.fong@i-med.ac.at.
¹³ Department of Hematology and Oncology, Medical University of Innsbruck, Innsbruck, Austria. guenther.gastl@i-med.ac.at.
¹⁴ Experimental Oncogenomics, Tyrolean Cancer Research Institute, Innsbruck, Austria. gerold.untergasser@i-med.ac.at.
¹⁵ Oncotyrol - Center for Personalized Cancer Medicine, Innsbruck, Austria. gerold.untergasser@i-med.ac.at.
¹⁶ Department of Hematology and Oncology, Medical University of Innsbruck, Innsbruck, Austria. gerold.untergasser@i-med.ac.at.

Abstract

Background: EpCAM is highly expressed on membrane of epithelial tumor cells and has been detected as soluble/secreted (sEpCAM) in serum of cancer patients. In this study we established an ELISA for in vitro diagnostics to measure sEpCAM concentrations in ascites. Moreover, we evaluated the influence of sEpCAM levels on catumaxomab (antibody)--dependent cellular cytotoxicity (ADCC).

Methods: Ascites specimens from cancer patients with positive (C+, n = 49) and negative (C-, n = 22) cytology and ascites of patients with liver cirrhosis (LC, n = 31) were collected. All cell-free plasma samples were analyzed for sEpCAM levels with a sandwich ELISA system established and validated by a human recombinant EpCAM standard for measurements in ascites as biological matrix. In addition, we evaluated effects of different sEpCAM concentrations on catumaxomab-dependent cell-mediated cytotoxicity (ADCC) with human peripheral blood mononuclear cells (PBMNCs) and human tumor cells.

Results: Our ELISA showed a high specificity for secreted EpCAM as determined by control HEK293FT cell lines stably expressing intracellular (EpICD), extracellular (EpEX) and the full-length protein (EpCAM) as fusion proteins. The lower limit of quantification was 200 pg/mL and the linear quantification range up to 5,000 pg/mL in ascites as biological matrix. Significant levels of sEpCAM were found in 39% of C+, 14% of C- and 13% of LC ascites samples. Higher concentrations of sEpCAM were detectable in C+ (mean: 1,015 pg/mL) than in C- (mean: 449 pg/mL; p = 0.04) or LC (mean: 326 pg/mL; p = 0.01). Soluble EpCAM concentration of 1 ng/mL significantly inhibited ADCC of PBMNCs on EpCAM overexpressing target cells.

Conclusion: Elevated concentrations of sEpCAM can be found in a subgroup of C+ and also in a small group of C- patients. We consider that sEpCAM levels in different tumor entities and individual patients should be evaluated prior to applying anti-EpCAM antibody-based cancer therapies, since sEpCAM neutralizes catumaxomab activity, making therapy less efficient.

Publication types

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

MeSH terms

Antibodies, Bispecific / pharmacology*
Antigens, Neoplasm / metabolism*
Ascites / metabolism*
Ascites / pathology*
Cell Adhesion Molecules / metabolism*
Cell Line, Tumor
Cell Proliferation / drug effects
Cytotoxicity, Immunologic
Epithelial Cell Adhesion Molecule
HEK293 Cells
Humans
Liver Cirrhosis / pathology
Neoplasms / pathology
Retrospective Studies

Substances

Antibodies, Bispecific
Antigens, Neoplasm
Cell Adhesion Molecules
EPCAM protein, human
Epithelial Cell Adhesion Molecule
catumaxomab