Digital Droplet PCR Is a Reliable Tool to Improve Minimal Residual Disease Stratification in Adult Philadelphia-Negative Acute Lymphoblastic Leukemia

被引:9
作者
Della Starza, Irene [1 ,3 ]
De Novi, Lucia A. [1 ]
Santoro, Alessandra [4 ]
Salemi, Domenico [4 ]
Spinelli, Orietta [5 ]
Tosi, Manuela [5 ]
Soscia, Roberta [1 ]
Paoloni, Francesca [3 ]
V. Cappelli, Luca V. [1 ]
Cavalli, Marzia [1 ]
Apicella, Valerio [1 ]
Bellomarino, Vittorio [1 ]
Di Lello, Eleonora [1 ]
Vitale, Antonella [1 ]
Vignetti, Marco [3 ]
Fabbiano, Francesco [4 ]
Rambaldi, Alessandro [5 ]
Bassan, Renato [6 ,7 ]
Guarini, Anna [1 ,2 ]
Chiaretti, Sabina [1 ,8 ]
Foa, Robin [8 ]
机构
[1] Sapienza Univ Rome, Dept Translat & Precis Med, Hematol, Rome, Italy
[2] Sapienza Univ Rome, Dept Mol Med, Rome, Italy
[3] GIMEMA Fdn, Rome, Italy
[4] Ospedali Riuniti Villa Sofia Cervello, Div Hematol & Bone Marrow Transplantat, Palermo, Italy
[5] ASST Papa Giovanni XXIII, Hematol & Bone Marrow Trasplant Unit, Bergamo, Italy
[6] Osped SS Giovanni & Paolo, Hematol Unit, Venice, Italy
[7] Osped Angelo, Venice, Italy
[8] Sapienza Univ Rome, Hematol, Via Benevento 6, I-00161 Rome, Italy
关键词
RECEPTOR GENE REARRANGEMENTS; TIME QUANTITATIVE PCR; CONCERTED ACTION; RQ-PCR; RELAPSE; PRIMERS; QUANTIFICATION; IMMUNOGLOBULIN; PROTOCOLS;
D O I
10.1016/j.jmoldx.2022.04.014
中图分类号
R36 [病理学];
学科分类号
100104 ;
摘要
Digital droplet PCR (ddPCR) is an implementation of conventional PCR, with the potential of overcoming some limitations of real-time quantitative PCR (RQ-PCR). To evaluate if ddPCR may improve the quan-tification of disease levels and refine patients' risk stratification, 116 samples at four time points from 44 (35 B-lineage and 9 T-lineage) adult Philadelphia-negative acute lymphoblastic leukemia patients enrolled in the GIMEMA LAL1913 protocol were analyzed by RQ-PCR and ddPCR. A concordance rate between RQ-PCR and ddPCR of 79% (P < 0.0001) was observed; discordances were identified in 21% of samples, with the majority being RQ-PCR-negative (NEG) or positive not quantifiable (PNQ). ddPCR significantly reduced the proportion of PNQ samplesd2.6% versus 14% (P Z 0.003)dand allowed disease quantifiability in 6.6% of RQ-PCR-NEG, increasing minimal residual disease quantification in 14% of samples. Forty-seven samples were also investigated by next-generation sequencing, which confirmed the ddPCR results in samples classified as RQ-PCR-PNQ or NEG. By reclassifying samples on the basis of the ddPCR results, a better event-free survival stratification of patients was observed compared to RQ-PCR; indeed, ddPCR captured more true-quantifiable samples, with five relapses occurring in three pa-tients who resulted RQ-PCR-PNQ/NEG but proved ddPCR positive quantifiable. At variance, no relapses were recorded in patients whose follow-up samples were RQ-PCR-PNQ but reclassified as ddPCR-NEG. A broader application of ddPCR in acute lymphoblastic leukemia clinical trials will help to improve patients' stratification.
引用
收藏
页码:893 / 900
页数:8
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