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使用液滴数字PCR分析神经母细胞瘤患者血浆中的拷贝数。

Using droplet digital PCR to analyze and copy number in plasma from patients with neuroblastoma.

作者信息

Lodrini Marco, Sprüssel Annika, Astrahantseff Kathy, Tiburtius Daniela, Konschak Robert, Lode Holger N, Fischer Matthias, Keilholz Ulrich, Eggert Angelika, Deubzer Hedwig E

机构信息

Department of Pediatric Hematology, Oncology and Stem Cell Transplantation, Charité-Universitätsmedizin Berlin, Berlin, Germany.

Translational Radiation Oncology Research Laboratory, Department of Radiooncology and Radiotherapy, Charité-Universitätsmedizin Berlin, Berlin, Germany.

出版信息

Oncotarget. 2017 Jul 7;8(49):85234-85251. doi: 10.18632/oncotarget.19076. eCollection 2017 Oct 17.

Abstract

The invasive nature of surgical biopsies deters sequential application, and single biopsies often fail to reflect tumor dynamics, intratumor heterogeneity and drug sensitivities likely to change during tumor evolution and treatment. Implementing molecular characterization of cell-free neuroblastoma-derived DNA isolated from blood plasma could improve disease assessment for treatment selection and monitoring of patients with high-risk neuroblastoma. We established droplet digital PCR (ddPCR) protocols for and copy number status in plasma from neuroblastoma patients. Our ddPCR protocol accurately discriminated between and amplification, gain and normal diploid status in a large panel of neuroblastoma cell lines, and discrepancies with reported and status were detected, including a high-level amplification in NB-1, a gain in SH-SY5Y, a high-level amplification in IMR-32 and gains in BE(2)-C, Kelly, SH-SY5Y and LAN-6. and status were also reliably determined from cell-free DNA derived from medium conditioned by the cell lines. and copy numbers of subcutaneous neuroblastoma xenograft tumors were accurately determined from cell-free DNA in the mouse blood plasma. In a final validation step, we accurately distinguished and copy numbers of the corresponding primary tumors using retrospectively collected blood plasma samples from 10 neuroblastoma patients. Our data justify the further development of molecular disease characterization using cell-free DNA in blood plasma from patients with neuroblastoma. This expanded molecular diagnostic palette may improve monitoring of disease progression including relapse and metastatic events as well as therapy success or failure in high-risk neuroblastoma patients.

摘要

手术活检的侵入性阻碍了其连续应用,而且单次活检往往无法反映肿瘤动态、肿瘤内异质性以及在肿瘤演变和治疗过程中可能发生变化的药物敏感性。对从血浆中分离出的无细胞神经母细胞瘤衍生DNA进行分子特征分析,可能会改善对高危神经母细胞瘤患者的疾病评估,以用于治疗选择和监测。我们建立了用于检测神经母细胞瘤患者血浆中 和 拷贝数状态的液滴数字PCR(ddPCR)方案。我们的ddPCR方案在一大组神经母细胞瘤细胞系中准确区分了 和 的扩增、增益和正常二倍体状态,并检测到与报道的 和 状态存在差异,包括NB-1中的高水平 扩增、SH-SY5Y中的 增益、IMR-32中的高水平 扩增以及BE(2)-C、Kelly、SH-SY5Y和LAN-6中的 增益。从细胞系条件培养基中获得的无细胞DNA也可靠地确定了 和 状态。从小鼠血浆中的无细胞DNA准确测定了皮下神经母细胞瘤异种移植瘤的 和 拷贝数。在最后的验证步骤中,我们使用从10例神经母细胞瘤患者回顾性收集的血浆样本,准确区分了相应原发肿瘤的 和 拷贝数。我们的数据证明了利用神经母细胞瘤患者血浆中的无细胞DNA进一步开展分子疾病特征分析的合理性。这种扩展的分子诊断方法可能会改善对疾病进展的监测,包括复发和转移事件,以及高危神经母细胞瘤患者的治疗成败。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/94e6/5689606/07f26d86ad9f/oncotarget-08-85234-g001.jpg

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