A single droplet digital PCR for ESR1 activating mutations detection in plasma

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Jeannot, Emmanuelle | Darrigues, Lauren | Michel, Marc | Stern, Marc Henri | Pierga, Jean Yves | Rampanou, Aurore | Melaabi, Samia | Benoist, Camille | Bièche, Ivan | Vincent-Salomon, Anne | El Ayachy, Radouane | Noret, Aurélien | Epaillard, Nicolas | Cabel, Luc | Bidard, François Clément | Proudhon, Charlotte

Edité par CCSD ; Nature Publishing Group [1987-....] -

International audience. Activating mutations in the estrogen receptor 1 (ESR1) gene confer resistance to aromatase inhibitors (AI), and may be targeted by selective estrogen receptor downregulators. We designed a multiplex droplet digital PCR (ddPCR), which combines a drop-off assay, targeting the clustered hotspot mutations found in exon 8, with an unconventional assay interrogating the E380Q mutation in exon 5. We assessed its sensitivity in vitro using synthetic oligonucleotides, harboring E380Q, L536R, Y537C, Y537N, Y537S, or D538G mutations. Further validation was performed on plasma samples from a prospective study and compared with next generation sequencing (NGS) data. The multiplex ESR1-ddPCR showed a high sensitivity with a limit of detection ranging from 0.07 to 0.19% in mutant allele frequency. The screening of plasma samples from patients with AI-resistant metastatic breast cancer identified ESR1 mutations in 29% of them, all mutations being confirmed by NGS. In addition, this test identifies patients harboring polyclonal alterations. Furthermore, the monitoring of circulating tumor DNA using this technique during treatment follow-up predicts the clinical benefit of palbociclib–fulvestrant. The multiplex ESR1-ddPCR detects, in a single reaction, the most frequent ESR1 activating mutations with good sensitivity. This method allows real-time liquid biopsy for ESR1 mutation monitoring in large cohorts of patients.

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