The Droplet Digital PCR: A New Valid Molecular Approach for the Assessment of B-RAF V600E Mutation in Hairy Cell Leukemia

Guerrini, Francesca; Paolicchi, Matteo; Ghio, Francesco; Ciabatti, Elena; Grassi, Susanna; Salehzadeh, Serena; Ercolano, Giacomo; Metelli, Maria Rita; Re, Marzia Del; Iovino, Lorenzo; Petrini, Iacopo; Carulli, Giovanni; Cecconi, Nadia; Rousseau, Martina; Cervetti, Giulia; Galimberti, Sara

doi:10.3389/fphar.2016.00363

Cited by 25 publications

(26 citation statements)

References 49 publications

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“…Although in a limited number of samples, it is worth to notice the absence of interlaboratory discordance when ddPCR was applied to brd samples. This is in line with previous studies showed that ddPCR and RQ exhibit a good correlation in MRD quantification in different diseases [16][17][18]27,28 ; moreover, in samples with low MRD levels, ddPCR appears able to identify a quantifiable disease more reliably than RQ and to discriminate very low MRD level from false positive samples. 32 Next-generation sequencing (NGS) has also been shown to represent an excellent tool for MRD detection in precursor and mature B-cell tumors.…”

Section: Discussionsupporting

confidence: 92%

“…ddPCR appears a promising tool for MRD monitoring. [16][17][18]27,28 Based on the dynamic nature of the method, ddPCR seems to be more accurate than RQ since (a) each sample is partitioned in thousands of droplets, representing thousands of independent PCR, and each droplet is analyzed individually; (b) small changes in fluorescence intensity are more readily detected; and (c) the ratio between target DNA molecules to PCR reagents is substantially higher. [29][30][31] Since February 2015, we have included also ddPCR in the QC rounds.…”

Section: Discussionmentioning

confidence: 99%

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Minimal residual disease (MRD) in non‐Hodgkin lymphomas: Interlaboratory reproducibility on marrow samples with very low levels of disease within the FIL (Fondazione Italiana Linfomi) MRD Network

Starza

Cavalli

Novi

et al. 2019

Hematological Oncology

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In 2009, the four laboratories of the Fondazione Italiana Linfomi (FIL) minimal residual disease (MRD) Network started a collaborative effort to harmonize and standardize their methodologies at the national level, performing quality control (QC) rounds for follicular lymphoma (FL) and mantle cell lymphoma (MCL) MRD assessment. In 16 QC rounds between 2010 and 2017, the four laboratories received 208 bone marrow (BM) samples (126 FL; 82 MCL); 187 were analyzed, according to the EuroMRD Consortium guidelines, by both nested (NEST) polymerase chain reaction (PCR) and real‐time quantitative (RQ) PCR for BCL2/IGH MBR or IGHV rearrangements. Here, we aimed at analyzing the samples that challenged the interlaboratory reproducibility and data interpretation. Overall, 156/187 BM samples (83%) were concordantly classified as NEST+/RQ+ or NEST−/RQ− by all the four laboratories. The remaining 31 samples (17%) resulted alternatively positive and negative in the interlaboratory evaluations, independently of the method and the type of rearrangement, and were defined “borderline” (brd) samples: 12 proved NEST brd/RQ brd, 7 NEST−/RQ brd, 10 NEST brd/RQ positive not quantifiable (PNQ), and 2 NEST brd/RQ−. Results did not change even increasing the number of replicates/sample. In 6/31 brd samples, droplet digital PCR (ddPCR) was tested and showed no interlaboratory discordance. Despite the high interlaboratory reproducibility in the MRD analysis obtained and maintained by the QC round strategy, samples with the lowest MRD levels can still represent a challenge: 17% (31/187) of our samples showed discordant results in interlaboratory assessments, with 6.4% (12/187) remained brd even applying the two methods. Thus, although representing a minority, brd samples are still problematic, especially when a clinically oriented interpretation of MRD results is required. Alternative, novel methods such as ddPCR and next‐generation sequencing have the potential to overcome the current limitations.

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Section: Discussionsupporting

confidence: 92%

Section: Discussionmentioning

confidence: 99%

Minimal residual disease (MRD) in non‐Hodgkin lymphomas: Interlaboratory reproducibility on marrow samples with very low levels of disease within the FIL (Fondazione Italiana Linfomi) MRD Network

Starza

Cavalli

Novi

et al. 2019

Hematological Oncology

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“…So far, only a few studies, afterwards described, report dPCR use for MRD monitoring in lymphoprolipherative disorders [ 23 , 42 , 43 , 44 , 45 , 46 , 47 ]. Actually, more progresses have been achieved by dPCR for MRD evaluation in other hematological malignancies.…”

Section: Digital Pcr For Mrd Monitoringmentioning

confidence: 99%

“…In a recent study, Guerrini F. et al [ 46 ] used droplet dPCR for the detection of B-RAF V600E mutation in HCL; MRD detection by this technique was significantly correlated to clinical status. Moreover, in this study, the authors compared the two quantitative methods showing a sensitivity of droplet dPCR more than half a log higher than qPCR, similar to the sensitivity levels reported for MYD88 L265P mutation detection; in fact, in WM patients, droplet dPCR reached a sensitivity of 5.0 × 10 −5 , compared to the 1.0 × 10 −3 achievable by ASO-PCR [ 53 ].…”

Section: Digital Pcr For Mrd Monitoringmentioning

confidence: 99%

New Molecular Technologies for Minimal Residual Disease Evaluation in B-Cell Lymphoid Malignancies

Dogliotti

Drandi

Genuardi

et al. 2018

JCM

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The clearance of malignant clonal cells significantly correlates with clinical outcomes in many hematologic malignancies. Accurate and high throughput tools for minimal residual disease (MRD) detection are needed to overcome some drawbacks of standard molecular techniques; such novel tools have allowed for higher sensitivity analyses and more precise stratification of patients, based on molecular response to therapy. In this review, we depict the recently introduced digital PCR and next-generation sequencing technologies, describing their current application for MRD monitoring in lymphoproliferative disorders. Moreover, we illustrate the feasibility of these new technologies to test less invasive and more patient-friendly tissues sources, such as “liquid biopsy”.

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“…MRD is the major cause of relapse in cancers [29]. Recently, ddPCR has been shown to have promise in MRD monitoring where assays with high sensitivity are [30] proposed that ddPCR would be applicable in the monitoring of MRD and follow-up of patients with Hairy cell leukemia, as it showed higher sensitivity in detecting B-RAF mutation compared with qPCR (0.005% vs. 0.025%). Moreover, the detection limit in B-RAF mutations was 0.0005% when ddPCR was combined with whole genome amplification [31].…”

Section: Cancer Progression and Treatment Response Monitoringmentioning

confidence: 99%

Application of Digital PCR in Detecting Human Diseases Associated Gene Mutation

Yu¹,

Shen²,

Jiang³

et al. 2017

Cell Physiol Biochem

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Gene mutation has been considered a research hotspot, and the rapid development of biomedicine has enabled significant advances in the evaluation of gene mutations. The advent of digital polymerase chain reaction (dPCR) elevates the detection of gene mutations to unprecedented levels of precision, especially in cancer-associated genes. dPCR has been utilized in the detection of tumor markers in cell-free DNA (cfDNA) samples from patients with different types of cancer in samples such as plasma, cerebrospinal fluid, urine and sputum, which confers significant value for dPCR in both clinical applications and basic research. Moreover, dPCR is extensively used in detecting pathogen mutations related to typical features of infectious diseases (e.g., drug resistance) and mutation status of heteroplasmic mitochondrial DNA, which determines the manifestation and progression of mtDNA-related diseases, as well as allows for the prenatal diagnosis of monogenic diseases and the assessment of the genome editing effects. Compared with real-time PCR (qPCR) and sequencing, the higher sensitivity and accuracy of dPCR indicates a great advantage in the detection of rare mutation. As a new technique, dPCR has some limitations, such as the necessity of highly allele-specific probes and a large sample volume. In this review, we summarize the application of dPCR in the detection of human disease-associated gene mutations.

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The Droplet Digital PCR: A New Valid Molecular Approach for the Assessment of B-RAF V600E Mutation in Hairy Cell Leukemia

Cited by 25 publications

References 49 publications

Minimal residual disease (MRD) in non‐Hodgkin lymphomas: Interlaboratory reproducibility on marrow samples with very low levels of disease within the FIL (Fondazione Italiana Linfomi) MRD Network

Minimal residual disease (MRD) in non‐Hodgkin lymphomas: Interlaboratory reproducibility on marrow samples with very low levels of disease within the FIL (Fondazione Italiana Linfomi) MRD Network

New Molecular Technologies for Minimal Residual Disease Evaluation in B-Cell Lymphoid Malignancies

Application of Digital PCR in Detecting Human Diseases Associated Gene Mutation

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