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Cell‐free DNA aneuploidy score as a dynamic early response marker in prostate cancer

恩扎鲁胺 前列腺癌 肿瘤科 内科学 医学 雄激素受体 生物标志物 卡巴齐塔塞尔 癌症 非整倍体 多西紫杉醇 比例危险模型 生物 雄激素剥夺疗法 染色体 遗传学 基因
作者
Khrystany T. Isebia,Anouk C. de Jong,Lisanne F. van Dessel,Vanja de Weerd,Corine M. Beaufort,Jean Helmijr,J. Alberto Nakauma-González,Job van Riet,Paul Hamberg,Daniël J. Vis,Michiel S. van der Heijden,Nick Beije,Martijn P. Lolkema,Teoman Deger,Saskia M. Wilting,Ronald de Wit,Maurice P.H.M. Jansen,John W.M. Martens
出处
期刊:Molecular Oncology [Wiley]
卷期号:19 (10): 2822-2832 被引量:1
标识
DOI:10.1002/1878-0261.13797
摘要

Cell‐free circulating tumor DNA (ctDNA) has emerged as a promising biomarker for response evaluation in metastatic castration‐resistant prostate cancer (mCRPC). The current study evaluated the modified fast aneuploidy screening test‐sequencing system (mFast‐SeqS), a quick, tumor‐agnostic and affordable ctDNA assay that requires a small input of DNA, to generate a genome‐wide aneuploidy (GWA) score in mCRPC patients, and correlated this to matched metastatic tumor biopsies. In this prospective multicenter study, GWA scores were evaluated from blood samples of 196 mCRPC patients prior to treatment (baseline) with taxanes (docetaxel and cabazitaxel) and androgen receptor signaling inhibitors (ARSI; abiraterone and enzalutamide), and from 74 mCRPC patients at an early timepoint during treatment (early timepoint; median 21 days). Z ‐scores per chromosome arm were tested for their association with tumor tissue genomic alterations. We found that a high tumor load in blood (GWA high ) at baseline was associated with poor response to ARSI [HR: 2.63 (95% CI: 1.86–3.72) P < 0.001] but not to taxanes. Interestingly, GWA high score at the early timepoint was associated with poor response to both ARSIs [HR: 6.73 (95% CI: 2.60–17.42) P < 0.001] and taxanes [2.79 (95% CI: 1.34–5.78) P = 0.006]. A significant interaction in Cox proportional hazards analyses was seen when combining GWA status and type of treatment (at baseline P = 0.008; early timepoint P = 0.018). In summary, detection of ctDNA in blood by mFast‐SeqS is cheap, fast and feasible, and could be used at different timepoints as a potential predictor for outcome to ARSI and taxane treatment in mCRPC.
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