Integrating extracellular vesicle and circulating cell‐free DNA analysis using a single plasma aliquot improves the detection of HER2 positivity in breast cancer patients

Author:

Mugoni Vera1ORCID,Ciani Yari1,Quaini Orsetta1,Tomasini Simone1,Notarangelo Michela1,Vannuccini Federico1,Marinelli Alessia1,Leonardi Elena2,Pontalti Stefano3,Martinelli Angela1,Rossetto Daniele1,Pesce Isabella1,Mansy Sheref S.1,Barbareschi Mattia2,Ferro Antonella3,Caffo Orazio3,Attard Gerhardt4,Vizio Dolores Di5,D'Agostino Vito Giuseppe1,Nardella Caterina1,Demichelis Francesca1ORCID

Affiliation:

1. Department of Cellular, Computational and Integrative Biology University of Trento Trento Italy

2. Unit of Surgical Pathology, Santa Chiara Hospital, APSS Trento Italy

3. Department of Medical Oncology Santa Chiara Hospital, APSS Trento Italy

4. University College London Cancer Institute London UK

5. Department of Surgery, Division of Cancer Biology and Therapeutics Cedars‐Sinai Medical Center Los Angeles California USA

Abstract

AbstractMulti‐analyte liquid biopsies represent an emerging opportunity for non‐invasive cancer assessment. We developed ONCE (One Aliquot for Circulating Elements), an approach for the isolation of extracellular vesicles (EV) and cell‐free DNA (cfDNA) from a single aliquot of blood. We assessed ONCE performance to classify HER2‐positive early‐stage breast cancer (BrCa) patients by combining EV‐associated RNA (EV‐RNA) and cfDNA signals on n = 64 healthy donors (HD) and non–metastatic BrCa patients. Specifically, we isolated EV‐enriched samples by a charge‐based (CB) method and investigated EV‐RNA and cfDNA by next‐generation sequencing (NGS) and by digital droplet PCR (ddPCR). Sequencing of cfDNA and EV‐RNA from HER2‐ and HER2+ patients demonstrated concordance with in situ molecular analyses of matched tissues. Combined analysis of the two circulating analytes by ddPCR showed increased sensitivity in ERBB2/HER2 detection compared to single nucleic acid components. Multi‐analyte liquid biopsy prediction performance was comparable to tissue‐based sequencing results from TCGA. Also, imaging flow cytometry analysis revealed HER2 protein on the surface of EV isolated from the HER2+ BrCa plasma, thus corroborating the potential relevance of studying EV as companion analyte to cfDNA. This data confirms the relevance of combining cfDNA and EV‐RNA for HER2 cancer assessment and supports ONCE as a valuable tool for multi‐analytes liquid biopsies’ clinical implementation.

Funder

Fondazione Cassa Di Risparmio Di Trento E Rovereto

Publisher

Wiley

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