Large-Scale Plasma Proteome Epitome Profiling is an Efficient Tool for the Discovery of Cancer Biomarkers

Jozsef Lazar; Peter Antal-Szalmas; Istvan Kurucz; Annamaria Ferenczi; Mihaly Jozsi; Ilona Tornyi; Monika Muller; Janos Tibor Fekete; John Lamont; Peter FitzGerald; Anna Gall-Debreceni; Janos Kadas; Andras Vida; Nadege Tardieu; Yann Kieffer; Anne Jullien; Mariana Guergova-Kuras; William Hempel; Andras Kovacs; Tamas Kardos; Nora Bittner; Eszter Csanky; Maria Szilasi; Gyorgy Losonczy; Klara Szondy; Gabriella Galffy; Edit Csada; Klara Szalontai; Attila Somfay; David Malka; Paul Cottu; Krisztina Bogos; Laszlo Takacs

doi:10.1016/j.mcpro.2023.100580

Large-Scale Plasma Proteome Epitome Profiling is an Efficient Tool for the Discovery of Cancer Biomarkers

Mol Cell Proteomics. 2023 Jul;22(7):100580. doi: 10.1016/j.mcpro.2023.100580. Epub 2023 May 20.

Authors

Jozsef Lazar¹, Peter Antal-Szalmas², Istvan Kurucz³, Annamaria Ferenczi⁴, Mihaly Jozsi⁵, Ilona Tornyi⁶, Monika Muller⁷, Janos Tibor Fekete⁸, John Lamont⁹, Peter FitzGerald⁹, Anna Gall-Debreceni⁴, Janos Kadas⁴, Andras Vida¹⁰, Nadege Tardieu¹¹, Yann Kieffer¹¹, Anne Jullien¹¹, Mariana Guergova-Kuras¹¹, William Hempel¹¹, Andras Kovacs¹², Tamas Kardos¹³, Nora Bittner¹³, Eszter Csanky¹⁴, Maria Szilasi¹³, Gyorgy Losonczy¹⁵, Klara Szondy¹⁵, Gabriella Galffy¹⁵, Edit Csada¹⁶, Klara Szalontai¹⁶, Attila Somfay¹⁷, David Malka¹⁸, Paul Cottu¹⁹, Krisztina Bogos²⁰, Laszlo Takacs²¹

Affiliations

¹ Biosystems International Kft., Debrecen, Hungary; Biosystems Immunolab Zrt., Debrecen, Hungary. Electronic address: jozsef.lazar@biosys-ilab.com.
² Biosystems Immunolab Zrt., Debrecen, Hungary; Department of Laboratory Medicine, Faculty of Medicine, University of Debrecen, Debrecen, Hungary.
³ Biosystems International Kft., Debrecen, Hungary; Biosystems Immunolab Zrt., Debrecen, Hungary.
⁴ Biosystems International Kft., Debrecen, Hungary.
⁵ Department of Immunology, ELTE Eötvös Loránd University, Budapest, Hungary; MTA-ELTE Complement Research Group, Eötvös Loránd Research Network (ELKH), Budapest, Hungary.
⁶ Biosystems Immunolab Zrt., Debrecen, Hungary; Department of Human Genetics, Faculty of Medicine, University of Debrecen, Debrecen, Hungary.
⁷ Adware Research Kft., Balatonfüred, Hungary.
⁸ Department of Bioinformatics, Semmelweis University, Budapest, Hungary.
⁹ Randox Laboratories Ltd, Crumlin, United Kingdom.
¹⁰ Department of Laboratory Medicine, Faculty of Medicine, University of Debrecen, Debrecen, Hungary.
¹¹ Biosystems International SAS, Evry, France.
¹² Biosystems Immunolab Zrt., Debrecen, Hungary.
¹³ Department of Pulmonology, Faculty of Medicine, University of Debrecen, Debrecen, Hungary.
¹⁴ Department of Pulmonology, Miskolc Semmelweis Hospital and University Hospital, Miskolc, Hungary.
¹⁵ Department of Pulmonology, Faculty of Medicine, Semmelweis University, Budapest, Hungary.
¹⁶ Csongrád County Hospital of Chest Diseases, Deszk, Hungary.
¹⁷ Department of Pulmonology, Faculty of Medicine, University of Szeged, Deszk, Hungary.
¹⁸ Department of Medical Oncology, Gustave Roussy, Villejuif, France.
¹⁹ Department of Medical Oncology, Institut Curie, Paris, France.
²⁰ National Koranyi Institute for Pulmonology, Budapest, Hungary.
²¹ Biosystems International Kft., Debrecen, Hungary; Biosystems Immunolab Zrt., Debrecen, Hungary; Department of Human Genetics, Faculty of Medicine, University of Debrecen, Debrecen, Hungary; Biosystems International SAS, Evry, France. Electronic address: laszlo.takacs@biosys-ilab.com.

Abstract

Current proteomic technologies focus on the quantification of protein levels, while little effort is dedicated to the development of system approaches to simultaneously monitor proteome variability and abundance. Protein variants may display different immunogenic epitopes detectable by monoclonal antibodies. Epitope variability results from alternative splicing, posttranslational modifications, processing, degradation, and complex formation and possesses dynamically changing availability of interacting surface structures that frequently serve as reachable epitopes and often carry different functions. Thus, it is highly likely that the presence of some of the accessible epitopes correlates with function under physiological and pathological conditions. To enable the exploration of the impact of protein variation on the immunogenic epitome first, here, we present a robust and analytically validated PEP technology for characterizing immunogenic epitopes of the plasma. To this end, we prepared mAb libraries directed against the normalized human plasma proteome as a complex natural immunogen. Antibody producing hybridomas were selected and cloned. Monoclonal antibodies react with single epitopes, thus profiling with the libraries is expected to profile many epitopes which we define by the mimotopes, as we present here. Screening blood plasma samples from control subjects (n = 558) and cancer patients (n = 598) for merely 69 native epitopes displayed by 20 abundant plasma proteins resulted in distinct cancer-specific epitope panels that showed high accuracy (AUC 0.826-0.966) and specificity for lung, breast, and colon cancer. Deeper profiling (≈290 epitopes of approximately 100 proteins) showed unexpected granularity of the epitope-level expression data and detected neutral and lung cancer-associated epitopes of individual proteins. Biomarker epitope panels selected from a pool of 21 epitopes of 12 proteins were validated in independent clinical cohorts. The results demonstrate the value of PEP as a rich and thus far unexplored source of protein biomarkers with diagnostic potential.

Keywords: biomarker; cancer; epitope; lung cancer; plasma epitom profiling; protein variants; proteoform.

Publication types

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

MeSH terms

Antibodies, Monoclonal / chemistry
Biomarkers, Tumor*
Epitopes
Humans
Neoplasms*
Proteome
Proteomics / methods

Substances

Biomarkers, Tumor
Proteome
Epitopes
Antibodies, Monoclonal