ASPYRE-Lung: validation of a simple, fast, robust and novel method for multi-variant genomic analysis of actionable NSCLC variants in FFPE tissue

Ryan T Evans; Elizabeth Gillon-Zhang; Julia N Brown; Katherine E Knudsen; Candace King; Amanda S Green; Ana-Luisa Silva; Justyna M Mordaka; Rebecca N Palmer; Alessandro Tomassini; Alejandra Collazos; Christina Xyrafaki; Iyelola Turner; Chau Ha Ho; Dilyara Nugent; Jinsy Jose; Simonetta Andreazza; Nicola D Potts; Kristine von Bargen; Eleanor R Gray; Magdalena Stolarek-Januszkiewicz; Aishling Cooke; Honey V Reddi; Barnaby W Balmforth; Robert J Osborne

doi:10.3389/fonc.2024.1420162

ASPYRE-Lung: validation of a simple, fast, robust and novel method for multi-variant genomic analysis of actionable NSCLC variants in FFPE tissue

Front Oncol. 2024 Sep 25:14:1420162. doi: 10.3389/fonc.2024.1420162. eCollection 2024.

Authors

Ryan T Evans¹, Elizabeth Gillon-Zhang¹, Julia N Brown¹, Katherine E Knudsen¹, Candace King¹, Amanda S Green¹, Ana-Luisa Silva², Justyna M Mordaka², Rebecca N Palmer², Alessandro Tomassini², Alejandra Collazos², Christina Xyrafaki², Iyelola Turner², Chau Ha Ho², Dilyara Nugent², Jinsy Jose², Simonetta Andreazza², Nicola D Potts², Kristine von Bargen², Eleanor R Gray², Magdalena Stolarek-Januszkiewicz², Aishling Cooke², Honey V Reddi¹, Barnaby W Balmforth¹, Robert J Osborne²

Affiliations

¹ Biofidelity Inc., Morrisville, NC, United States.
² Biofidelity Ltd., Cambridge, United Kingdom.

Abstract

Introduction: Genomic variant testing of tumors is a critical gateway for patients to access the full potential of personalized oncology therapeutics. Current methods such as next-generation sequencing are costly and challenging to interpret, while PCR assays are limited in the number of variants they can cover. We developed ASPYRE^® (Allele-Specific PYrophosphorolysis REaction) technology to address the urgent need for rapid, accessible and affordable diagnostics informing actionable genomic target variants of a given cancer. The targeted ASPYRE-Lung panel for non-small cell carcinoma covers 114 variants in 11 genes (ALK, BRAF, EGFR, ERBB2, KRAS, RET, ROS1, MET & NTRK1/2/3) to robustly inform clinical management. The assay detects single nucleotide variants, insertions, deletions, and gene fusions from tissue-derived DNA and RNA simultaneously.

Methods: We tested the limit of detection, specificity, analytical accuracy and analytical precision of ASPYRE-Lung using FFPE lung tissue samples from patients with non-small cell lung carcinoma, variant-negative FFPE tissue from healthy donors, and FFPE-based contrived samples with controllable variant allele fractions.

Results: The sensitivity of ASPYRE-Lung was determined to be ≤ 3% variant allele fraction for single nucleotide variants and insertions or deletions, 100 copies for fusions, and 200 copies for MET exon 14 skipping. The specificity was 100% with no false positive results. The analytical accuracy test yielded no discordant calls between ASPYRE-Lung and expected results for clinical samples (via orthogonal testing) or contrived samples, and results were replicable across operators, reagent lots, runs, and real-time PCR instruments with a high degree of precision.

Conclusions: The technology is simple and fast, requiring only four reagent transfer steps using standard laboratory equipment (PCR and qPCR instruments) with analysis via a cloud-based algorithm. The ASPYRE-Lung assay has the potential to be transformative in facilitating access to rapid, actionable molecular profiling of tissue for patients with non-small cell carcinoma.

Keywords: NSCLC; assay validation; molecular diagnosis; precision oncology; pyrophosphorolysis; targeted panel.

Copyright © 2024 Evans, Gillon-Zhang, Brown, Knudsen, King, Green, Silva, Mordaka, Palmer, Tomassini, Collazos, Xyrafaki, Turner, Ho, Nugent, Jose, Andreazza, Potts, von Bargen, Gray, Stolarek-Januszkiewicz, Cooke, Reddi, Balmforth and Osborne.

Grants and funding

The author(s) declare financial support was received for the research, authorship, and/or publication of this article. Funding for this work was provided by Biofidelity Ltd.