Diagnostics (Jun 2023)

Development of a Detection System for <i>ESR1</i> Mutations in Circulating Tumour DNA Using PNA-LNA-Mediated PCR Clamping

  • Yuki Kojima,
  • Emi Noguchi,
  • Tomomi Yoshino,
  • Shigehiro Yagishita,
  • Shu Yazaki,
  • Hitomi S. Okuma,
  • Tadaaki Nishikawa,
  • Maki Tanioka,
  • Kazuki Sudo,
  • Tatsunori Shimoi,
  • Ayaka Kazama,
  • Hiroshi Terasaki,
  • Sachiro Asano,
  • Yasuhiro Fujiwara,
  • Akinobu Hamada,
  • Kenji Tamura,
  • Kan Yonemori

DOI
https://doi.org/10.3390/diagnostics13122040
Journal volume & issue
Vol. 13, no. 12
p. 2040

Abstract

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Although circulating tumour DNA (ctDNA)-based next-generation sequencing (NGS) is a less invasive method for assessing ESR1 mutations that are essential mechanisms of endocrine therapy resistance in patients with oestrogen receptor-positive breast cancer, adequate amounts of DNA are required to assess polyclonal ESR1 mutations. By combining a peptide nucleic acid and locked nucleic acid polymerase chain reaction (PNA-LNA PCR) clamping assay, we have developed a novel detection system to screen for polyclonal ESR1 mutations in ctDNA. A validation assay was prospectively performed on clinical samples and compared with the NGS results. The PNA-LNA PCR clamp assay was validated using six and four blood samples in which ESR1 mutations were detected by NGS and no mutations were detected, respectively. The PNA-LNA assay results were comparable with those of NGS. We prospectively assessed the concordance between the PNA-LNA PCR clamp method and NGS. Using the PNA-LNA PCR clamp method, ESR1 mutations were detected in 5 out of 18 samples, including those in which mutations were not detected by NGS due to small amounts of ctDNA. The PNA-LNA PCR clamping method is a highly sensitive and minimally invasive assay for polyclonal ESR1 mutation detection in the ctDNA of patients with breast cancer.

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