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通过液滴数字 PCR 与实时 PCR 检测和定量嵌合抗原受体转基因拷贝数。

Detection and Quantification of Chimeric Antigen Receptor Transgene Copy Number by Droplet Digital PCR versus Real-Time PCR.

机构信息

Department of Hematology, Tongji Hospital, Tongji Medical College, Huazhong University of Science and Technology, Wuhan, People's Republic of China.

Department of Hematology, Tongji Hospital, Tongji Medical College, Huazhong University of Science and Technology, Wuhan, People's Republic of China.

出版信息

J Mol Diagn. 2020 May;22(5):699-707. doi: 10.1016/j.jmoldx.2020.02.007.

DOI:10.1016/j.jmoldx.2020.02.007
PMID:32409121
Abstract

Chimeric antigen receptor (CAR) T-cell immunotherapy is a new strategy for the treatment of refractory B-cell malignancies; therefore, the rapid and accurate quantification of CAR transgene copy number is essential. Real-time PCR was used for quantifying the copy number of chimeric antigen receptor transgene. Droplet digital PCR (ddPCR) is an absolute quantification method that does not require a standard curve. In this study, key performance parameters of the ddPCR and real-time PCR methods were assessed, including linearity, detection range, the lower limit of detection, repeatability, reproducibility, and accuracy, using a series of gradient diluted standards and clinical peripheral blood samples from CAR T-cell patients. The two platforms showed a good correlation for the standards (Pearson R = 0.9966; P < 0.0001) and clinical samples (Pearson R = 0.8952; P < 0.0001), and both showed good linearity (R = 0.9996 for ddPCR; R = 0.9984 for real-time PCR) over the detection range. Compared with real-time PCR, ddPCR showed lower intra-assay and interassay CVs for the series of diluted standards, which indicated ddPCR has better repeatability and reproducibility. The limit of detection of ddPCR was lower compared with that of real-time PCR. The combined results suggest that ddPCR is a more promising tool for the detection and quantification of the chimeric antigen receptor transgene copy number.

摘要

嵌合抗原受体 (CAR) T 细胞免疫疗法是治疗难治性 B 细胞恶性肿瘤的一种新策略;因此,快速准确地定量 CAR 转基因拷贝数至关重要。实时 PCR 用于定量嵌合抗原受体转基因的拷贝数。微滴式数字 PCR (ddPCR) 是一种绝对定量方法,不需要标准曲线。在这项研究中,使用一系列梯度稀释的标准品和 CAR T 细胞患者的临床外周血样本,评估了 ddPCR 和实时 PCR 方法的关键性能参数,包括线性、检测范围、检测下限、重复性、重现性和准确性。两种平台对标准品的相关性良好(Pearson R=0.9966;P<0.0001)和临床样本(Pearson R=0.8952;P<0.0001),并且在检测范围内都表现出良好的线性(ddPCR 的 R=0.9996;实时 PCR 的 R=0.9984)。与实时 PCR 相比,ddPCR 对系列稀释标准品的内和间测定 CV 较低,这表明 ddPCR 具有更好的重复性和重现性。ddPCR 的检测限低于实时 PCR。综合结果表明,ddPCR 是一种更有前途的检测和定量嵌合抗原受体转基因拷贝数的工具。

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