3143:监测ER阳性(POS)/HER2阴性(NEG)晚期乳腺癌内分泌治疗期间循环肿瘤细胞(CTC)和循环肿瘤DNA (ctDNA)基因组改变:AZD9496口服SERD I期试验的相关研究

Q3 Biochemistry, Genetics and Molecular Biology Tumor Biology Pub Date : 2021-07-01 DOI:10.1158/1538-7445.AM2021-3143
A. Cani, Emily M Dolce, Elizabeth P. Darga, K. Hu, Martha E. Brown, C. Liu, J. Pierce, K. Bradbury, K. Aung, G. Schiavon, Danielle Carroll, T. Carr, T. Klinowska, J. Lindemann, G. Marshall, V. Rowlands, E. Harrington, J. Barrett, A. Armstrong, R. Baird, E. Hamilton, S. Im, K. Jhaveri, M. Patel, C. Dive, S. Tomlins, A. Udager, D. Hayes, C. Paoletti
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Patients and Methods: Individual CTC and ctDNA were obtained at different time points from patients with advanced ER POS/HER2 NEG breast cancer enrolled in a Phase I trial of AZD9496, an oral selective estrogen receptor degrader (SERD) ET. The CTC, purified using tandem CellSearch®/DepArray™ technologies, were genomically profiled by DNA single cell next generation sequencing (scNGS). Plasma ctDNA was isolated from blood collected in Streck BCT tubes. Genomic profiling was performed by targeted gene panel scNGS for CTC and ddPCR for ERα gene (ESR1) mutations in ctDNA. Results: 123 high-quality CTCs from 12 patients profiled by scNGS showed 100% concordance with ctDNA in detection of driver ESR1 somatic mutations. CTC scNGS additionally revealed extensive intra-patient heterogeneity of driver alterations, that would have been unresolvable by bulk ctDNA profiling, including separate subclonal CTC populations emerging within the same patient. ScNGS revealed potential opportunities for targeted therapies in 73% of patients, directed at alterations in PIK3CA, FGFR2, KIT and BRAF, at times present as 2 or more targets in the same or different cell populations. In one patient, an emergent, distinct, BRAF p.V600E targetable alteration was detected in a subpopulation of CTCs collected at the progression time point but not at baseline. Conclusion: Serial monitoring of CTC and ctDNA genomic alterations is feasible and should enable real-time tracking of response/progression, tumor evolution and opportunities for precision medicine interventions. Citation Format: Andi K. Cani, Emily M. Dolce, Elizabeth P. Darga, Kevin Hu, Martha Brown, Chia-Jen Liu, Jackie Pierce, Kieran Bradbury, Kimberly Aung, Gaia Schiavon, Danielle Carroll, T. H. Carr, Teresa Klinowska, Justin Lindemann, Gayle Marshall, Vicky Rowlands, Elizabeth A. Harrington, J. Barrett, Anne Armstrong, Richard Baird, Erika Hamilton, Seock-Ah Im, Komal Jhaveri, Manish R. Patel, Caroline Dive, Scott A. Tomlins, Aaron M. Udager, Daniel F. Hayes, Costanza Paoletti. Monitoring circulating tumor cell (CTC) and circulating tumor DNA (ctDNA) genomic alterations in ER positive (POS)/HER2 negative (NEG) advanced breast cancer during endocrine therapy: correlative study of AZD9496 oral SERD phase I trial [abstract]. In: Proceedings of the American Association for Cancer Research Annual Meeting 2021; 2021 Apr 10-15 and May 17-21. 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引用次数: 0

摘要

目的:绝大多数晚期ER POS乳腺癌最终对内分泌(ET)和其他疗法停止反应,导致致命疾病的演变。然而,及时监测与组织活检反应/进展相关的分子事件在逻辑上是困难的。在这种情况下,液体活检的使用,如CTC和ctDNA,最近引起了人们的兴趣。患者和方法:从参与口服选择性雌激素受体降解剂(SERD)AZD9496的I期试验的晚期ER POS/HER2 NEG乳腺癌症患者中,在不同时间点获得单独的CTC和ctDNA™ 技术,通过DNA单细胞下一代测序(scNGS)进行基因组分析。从Streck BCT试管中采集的血液中分离血浆ctDNA。通过CTC的靶向基因组scNGS和ctDNA中ERα基因(ESR1)突变的ddPCR进行基因组分析。结果:来自12名scNGS患者的123个高质量CTC在检测驱动ESR1体细胞突变方面与ctDNA显示100%一致。CTC scNGS还揭示了驱动因素改变的广泛患者内异质性,这可能无法通过大量ctDNA分析来解决,包括在同一患者中出现的单独的亚克隆CTC群体。ScNGS在73%的患者中揭示了靶向治疗的潜在机会,针对PIK3CA、FGFR2、KIT和BRAF的改变,有时在相同或不同的细胞群中作为2个或多个靶点存在。在一名患者中,在进展时间点而不是基线收集的CTC亚群中检测到一种突发的、独特的BRAF p.V600E靶向性改变。结论:CTC和ctDNA基因组改变的连续监测是可行的,应该能够实时跟踪反应/进展、肿瘤演变和精准医学干预的机会。引文格式:Andi K.Cani、Emily M.Dolce、Elizabeth P.Darga、Kevin Hu、Martha Brown、Chia Jen Liu、Jackie Pierce、Kieran Bradbury、Kimberly Aung、Gaia Schiavon、Danielle Carroll、T.H.Carr、Teresa Klinowska、Justin Lindemann、Gayle Marshall、Vicky Rowlands、Elizazabeth A.Harrington、J.Barrett、Anne Armstrong、Richard Baird、Erika Hamilton、Seock Ah Im、Komal Jhaveri、Manish R.Patel,Caroline Dive、Scott A.Tomlins、Aaron M.Udager、Daniel F.Hayes、Costanza Paoletti。内分泌治疗期间监测ER阳性(POS)/HER2阴性(NEG)晚期癌症循环肿瘤细胞(CTC)和循环肿瘤DNA(ctDNA)基因组变化:AZD9496口服SERD I期试验的相关性研究[摘要]。在:美国癌症研究协会2021年会论文集;2021年4月10-15日和5月17-21日。费城(PA):AACR;癌症研究2021;81(13_Suppl):摘要编号3143。
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Abstract 3143: Monitoring circulating tumor cell (CTC) and circulating tumor DNA (ctDNA) genomic alterations in ER positive (POS)/HER2 negative (NEG) advanced breast cancer during endocrine therapy: correlative study of AZD9496 oral SERD phase I trial
Purpose: The vast majority of advanced ER POS breast cancers eventually cease responding to endocrine (ET) and other therapies leading to evolution of lethal disease. However, timely monitoring of the molecular events associated with response/progression in tissue biopsies is logistically difficult. The use of liquid biopsies, such as CTC and ctDNA, in this context has been of recent interest. Patients and Methods: Individual CTC and ctDNA were obtained at different time points from patients with advanced ER POS/HER2 NEG breast cancer enrolled in a Phase I trial of AZD9496, an oral selective estrogen receptor degrader (SERD) ET. The CTC, purified using tandem CellSearch®/DepArray™ technologies, were genomically profiled by DNA single cell next generation sequencing (scNGS). Plasma ctDNA was isolated from blood collected in Streck BCT tubes. Genomic profiling was performed by targeted gene panel scNGS for CTC and ddPCR for ERα gene (ESR1) mutations in ctDNA. Results: 123 high-quality CTCs from 12 patients profiled by scNGS showed 100% concordance with ctDNA in detection of driver ESR1 somatic mutations. CTC scNGS additionally revealed extensive intra-patient heterogeneity of driver alterations, that would have been unresolvable by bulk ctDNA profiling, including separate subclonal CTC populations emerging within the same patient. ScNGS revealed potential opportunities for targeted therapies in 73% of patients, directed at alterations in PIK3CA, FGFR2, KIT and BRAF, at times present as 2 or more targets in the same or different cell populations. In one patient, an emergent, distinct, BRAF p.V600E targetable alteration was detected in a subpopulation of CTCs collected at the progression time point but not at baseline. Conclusion: Serial monitoring of CTC and ctDNA genomic alterations is feasible and should enable real-time tracking of response/progression, tumor evolution and opportunities for precision medicine interventions. Citation Format: Andi K. Cani, Emily M. Dolce, Elizabeth P. Darga, Kevin Hu, Martha Brown, Chia-Jen Liu, Jackie Pierce, Kieran Bradbury, Kimberly Aung, Gaia Schiavon, Danielle Carroll, T. H. Carr, Teresa Klinowska, Justin Lindemann, Gayle Marshall, Vicky Rowlands, Elizabeth A. Harrington, J. Barrett, Anne Armstrong, Richard Baird, Erika Hamilton, Seock-Ah Im, Komal Jhaveri, Manish R. Patel, Caroline Dive, Scott A. Tomlins, Aaron M. Udager, Daniel F. Hayes, Costanza Paoletti. Monitoring circulating tumor cell (CTC) and circulating tumor DNA (ctDNA) genomic alterations in ER positive (POS)/HER2 negative (NEG) advanced breast cancer during endocrine therapy: correlative study of AZD9496 oral SERD phase I trial [abstract]. In: Proceedings of the American Association for Cancer Research Annual Meeting 2021; 2021 Apr 10-15 and May 17-21. Philadelphia (PA): AACR; Cancer Res 2021;81(13_Suppl):Abstract nr 3143.
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来源期刊
Tumor Biology
Tumor Biology 医学-肿瘤学
CiteScore
5.40
自引率
0.00%
发文量
18
审稿时长
1 months
期刊介绍: Tumor Biology is a peer reviewed, international journal providing an open access forum for experimental and clinical cancer research. Tumor Biology covers all aspects of tumor markers, molecular biomarkers, tumor targeting, and mechanisms of tumor development and progression. Specific topics of interest include, but are not limited to: Pathway analyses, Non-coding RNAs, Circulating tumor cells, Liquid biopsies, Exosomes, Epigenetics, Cancer stem cells, Tumor immunology and immunotherapy, Tumor microenvironment, Targeted therapies, Therapy resistance Cancer genetics, Cancer risk screening. Studies in other areas of basic, clinical and translational cancer research are also considered in order to promote connections and discoveries across different disciplines. The journal publishes original articles, reviews, commentaries and guidelines on tumor marker use. All submissions are subject to rigorous peer review and are selected on the basis of whether the research is sound and deserves publication. Tumor Biology is the Official Journal of the International Society of Oncology and BioMarkers (ISOBM).
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