Insights on Droplet Digital PCR–Based Cellular Kinetics and Biodistribution Assay Support for CAR-T Cell Therapy

Sugimoto, Hiroshi; Chen, Susan; Minembe, Jean-Pierre; Chouitar, Johara; He, Xingyue; Wang, Haiqing; Fang, Xiaodong; Qian, Mark G.

doi:10.1208/s12248-021-00560-6

Cited by 18 publications

(19 citation statements)

References 23 publications

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“…Currently, clonal kinetics as well as in vivo distribution of CAR-T cells after re-infusion are topics of research. 16 , 35 , 36 Analyzing blood cells by flow cytometry and quantification of genomic DNA in peripheral blood mononuclear cells are the current standards to quantify CAR-T cells during treatment. Assay-specific limitations in qPCR analysis are adapted and under investigation.…”

Section: Discussionmentioning

confidence: 99%

“… 12 , 14 The handling of qPCR and ddPCR data is currently discussed, because multiple factors influence the amount and composition of cellular (genomic) DNA in patients' blood samples during CAR-T therapy. 15 , 16 …”

Section: Introductionmentioning

confidence: 99%

“…Following re-infusion, CAR-T cells distribute into various body areas and actively migrate into both tumor stroma and lymph nodes. 16 It is unknown whether loss of detectable CAR-T cells in blood samples corresponds to a loss of CAR-T cells due to apoptosis by cellular exhaustion or if it reflects cell sequestration in targeted tissues. Currently, studies investigating the biology of CAR-T cells following therapeutic administration are mainly focused on cellular samples.…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Quantification of cell-free DNA for the analysis of CD19-CAR-T cells during lymphoma treatment

Mika

Thomson

Nilius‐Eliliwi

et al. 2021

Molecular Therapy - Methods & Clinical Development

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Quantification of cell-free DNA for the analysis of CD19-CAR-T cells during lymphoma treatment

Mika

Thomson

Nilius‐Eliliwi

et al. 2021

Molecular Therapy - Methods & Clinical Development

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“…EC was added to all samples. DNA extraction from the calibration standard samples was conducted according to the method reported by Sugimoto et al (19), with minor modifications. DNA was extracted from 200 μL tissue homogenate or 50 μL blood using the KingFisher™ Flex system (MagMAX_Ultra2_200μL_Flex and MagMAXUltra 2TissueV).…”

Section: Optimization Of Dna Extraction Methodsmentioning

confidence: 99%

“…Droplet digital (dd) PCR runs reactions to the endpoint in partitioned individual droplets (19)(20)(21). The positive and negative droplets are divided based on droplet fluorescence, and DNA copy number is determined based on Poisson statistics.…”

Section: Introductionmentioning

confidence: 99%

Novel Cell Quantification Method Using a Single Surrogate Calibration Curve Across Various Biological Samples

Nakayama

Yamamoto

Hirabayashi

2023

AAPS J

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Quantitative polymerase chain reaction (qPCR) is generally used to quantify transplanted cell therapy products in biological samples. As the matrix effects on PCR amplification and variability in DNA recovery from biological samples are well-known limitations that hinder the assay’s performance, a calibration curve is conventionally established for each matrix. Droplet digital PCR (ddPCR) is based on the endpoint assay and advantageous in avoiding matrix effects. Moreover, the use of an external control gene may correct assay fluctuations to minimize the effects caused by inconsistent DNA recovery. In this study, we aimed to establish a novel and robust ddPCR method capable of quantifying human cells across various mouse biological samples using a single surrogate calibration curve in combination with an external control gene and DNA recovery normalization. Acceptable accuracy and precision were observed for quality control samples from different tissues, indicating the excellent quantitative and versatile potential of the developed method. Furthermore, the established method enabled the evaluation of human CD8+ T cell biodistribution in immunodeficient mice. Our findings provide new insights into the use of ddPCR-based quantification methods in biodistribution studies of cell therapy products. Graphical Abstract

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Bioanalytical Methods for Characterization of CAR‐T Cellular Kinetics: Comparison of PCR Assays and Matrices

Masilamani

Jawa

Dai

et al. 2023

Clin Pharma and Therapeutics

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Recently, multiple chimeric antigen receptor T‐cell (CAR‐T)‐based therapies have been approved for treating hematological malignancies, targeting CD19 and B‐cell maturation antigen. Unlike protein or antibody therapies, CAR‐T therapies are “living cell” therapies whose pharmacokinetics are characterized by expansion, distribution, contraction, and persistence. Therefore, this unique modality requires a different approach for quantitation compared with conventional ligand binding assays implemented for most biologics. Cellular (flow cytometry) or molecular assays (polymerase chain reaction (PCR)) can be deployed with each having unique advantages and disadvantages. In this article, we describe the molecular assays utilized: quantitative PCR (qPCR), which was the initial platform used to estimate transgene copy numbers and more recently droplet digital PCR (ddPCR) which quantitates the absolute copy numbers of CAR transgene. The comparability of the two methods in patient samples and of each method across different matrices (isolated CD3+ T‐cells or whole blood) was also performed. The results show a good correlation between qPCR and ddPCR for the amplification of same gene in clinical samples from a CAR‐T therapy trial. In addition, our studies show that the qPCR‐based amplification of transgene levels was well‐correlated, independent of DNA sources (either CD3+ T‐cells or whole blood). Our results also highlight that ddPCR can be a better platform for monitoring samples at the early phase of CAR‐T dosing prior to expansion and during long‐term monitoring as they can detect samples with very low copy numbers with high sensitivity, in addition to easier implementation and sample logistics.

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Insights on Droplet Digital PCR–Based Cellular Kinetics and Biodistribution Assay Support for CAR-T Cell Therapy

Cited by 18 publications

References 23 publications

Quantification of cell-free DNA for the analysis of CD19-CAR-T cells during lymphoma treatment

Quantification of cell-free DNA for the analysis of CD19-CAR-T cells during lymphoma treatment

Novel Cell Quantification Method Using a Single Surrogate Calibration Curve Across Various Biological Samples

Bioanalytical Methods for Characterization of CAR‐T Cellular Kinetics: Comparison of PCR Assays and Matrices

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