Comparison of Circulating Tumor DNA Assays for Molecular Residual Disease Detection in Early-Stage Triple-Negative Breast Cancer.

Coakley, Maria; Villacampa, Guillermo; Sritharan, Prithika; Swift, Claire; Dunne, Kathryn; Kilburn, Lucy; Goddard, Katie; Pipinikas, Christodoulos; Rojas, Patricia; Emmett, Warren; Hall, Peter; Harper-Wynne, Catherine; Hickish, Tamas; Macpherson, Iain; Okines, Alicia; Wardley, Andrew; Wheatley, Duncan; Waters, Simon; Palmieri, Carlo; Winter, Matthew; Cutts, Rosalind J; Garcia-Murillas, Isaac; Bliss, Judith; Turner, Nicholas C

Coakley, Maria; Villacampa, Guillermo; Sritharan, Prithika; Swift, Claire; Dunne, Kathryn; Kilburn, Lucy; Goddard, Katie; Pipinikas, Christodoulos; Rojas, Patricia; Emmett, Warren; Hall, Peter; Harper-Wynne, Catherine; Hickish, Tamas; Macpherson, Iain; Okines, Alicia; Wardley, Andrew; Wheatley, Duncan; Waters, Simon; Palmieri, Carlo; Winter, Matthew; Cutts, Rosalind J; Garcia-Murillas, Isaac; Bliss, Judith; Turner, Nicholas C.

Afiliação

Coakley M; Breast Cancer Now Research Centre, The Institute of Cancer Research, London, United Kingdom.
Villacampa G; Clinical Trials and Statistics Unit, The Institute of Cancer Research, London, United Kingdom.
Sritharan P; Breast Cancer Now Research Centre, The Institute of Cancer Research, London, United Kingdom.
Swift C; Ralph Lauren Centre for Breast Cancer Research, London, United Kingdom.
Dunne K; Ralph Lauren Centre for Breast Cancer Research, London, United Kingdom.
Kilburn L; Clinical Trials and Statistics Unit, The Institute of Cancer Research, London, United Kingdom.
Goddard K; Clinical Trials and Statistics Unit, The Institute of Cancer Research, London, United Kingdom.
Pipinikas C; NeoGenomics Ltd, Glenn Berge Building, Babraham Research Park, Cambridge, United Kingdom.
Rojas P; NeoGenomics Ltd, Glenn Berge Building, Babraham Research Park, Cambridge, United Kingdom.
Emmett W; NeoGenomics Ltd, Glenn Berge Building, Babraham Research Park, Cambridge, United Kingdom.
Hall P; University of Edinburgh, Edinburgh, United Kingdom.
Harper-Wynne C; Maidstone Hospital, Maidstone and Tunbridge Wells NHS Trust, Maidstone, United Kingdom.
Hickish T; University Hospitals Dorset NHS Foundation Trust, Bournemouth, United Kingdom.
Macpherson I; The Beatson West of Scotland Cancer Centre, Glasgow.
Okines A; Breast Unit, Royal Marsden Hospital, London, United Kingdom.
Wardley A; Outreach Research & Innovation Group Ltd, Manchester, United Kingdom.
Wheatley D; Royal Cornwall Hospitals NHS Trust, Truro, United Kingdom.
Waters S; Velindre Cancer Centre, Velindre University NHS Trust, Cardiff, United Kingdom.
Palmieri C; Clatterbridge Cancer Centre NHS Foundation Trust, Liverpool, United Kingdom.
Winter M; Weston Park Cancer Centre, Sheffield Teaching Hospitals NHS Foundation Trust, Sheffield, United Kingdom.
Cutts RJ; Breast Cancer Now Research Centre, The Institute of Cancer Research, London, United Kingdom.
Garcia-Murillas I; Breast Cancer Now Research Centre, The Institute of Cancer Research, London, United Kingdom.
Bliss J; Clinical Trials and Statistics Unit, The Institute of Cancer Research, London, United Kingdom.
Turner NC; Breast Cancer Now Research Centre, The Institute of Cancer Research, London, United Kingdom.

Clin Cancer Res ; 30(4): 895-903, 2024 02 16.

Article em En | MEDLINE | ID: mdl-38078899

ABSTRACT

ABSTRACT

PURPOSE:

Detection of circulating tumor DNA (ctDNA) in patients who have completed treatment for early-stage breast cancer is associated with a high risk of relapse, yet the optimal assay for ctDNA detection is unknown. EXPERIMENTAL

DESIGN:

The cTRAK-TN clinical trial prospectively used tumor-informed digital PCR (dPCR) assays for ctDNA molecular residual disease (MRD) detection in early-stage triple-negative breast cancer. We compared tumor-informed dPCR assays with tumor-informed personalized multimutation sequencing assays in 141 patients from cTRAK-TN.

RESULTS:

MRD was first detected by personalized sequencing in 47.9% of patients, 0% first detected by dPCR, and 52.1% with both assays simultaneously (P < 0.001; Fisher exact test). The median lead time from ctDNA detection to relapse was 6.1 months with personalized sequencing and 3.9 months with dPCR (P = 0.004, mixed-effects Cox model). Detection of MRD at the first time point was associated with a shorter time to relapse compared with detection at subsequent time points (median lead time 4.2 vs. 7.1 months; P = 0.02).

CONCLUSIONS:

Personalized multimutation sequencing assays have potential clinically important improvements in clinical outcome in the early detection of MRD.

Assuntos

DNA Tumoral Circulante; Neoplasias de Mama Triplo Negativas; Humanos; DNA Tumoral Circulante/genética; Neoplasias de Mama Triplo Negativas/diagnóstico; Neoplasias de Mama Triplo Negativas/genética; Recidiva Local de Neoplasia/patologia; Recidiva; Biomarcadores Tumorais/genética; Neoplasia Residual/diagnóstico; Neoplasia Residual/genética

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Texto completo: 1 Base de dados: MEDLINE Assunto principal: Neoplasias de Mama Triplo Negativas / DNA Tumoral Circulante Limite: Humans Idioma: En Revista: Clin Cancer Res Assunto da revista: NEOPLASIAS Ano de publicação: 2024 Tipo de documento: Article País de afiliação: Reino Unido

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