Quality Control of Flow Cytometry Data Analysis for Evaluation of Minimal Residual Disease in Bone Marrow From Acute Leukemia Patients During Treatment

Björklund, Elisabet; Matinlauri, Irma; Tierens, Anne; Axelsson, Susanne; Forestier, Erik; Jacobsson, Stefan; Ahlberg, Asa Jeppsson; Kauric, Goran; Mäntymaa, Pentti; Osnes, Liv; Penttilä, Tarja-Leena; Marquart, Hanne Vibeke; Savolainen, Eeva‐Riitta; Siitonen, Sanna; Torikka, Kerstin; Mazur, Joanna; Porwit, Anna

doi:10.1097/mph.0b013e3181a1c0e8

Cited by 22 publications

(28 citation statements)

References 22 publications

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“…Modulation of several markers is another confounding variable important for MRD analysis as we have seen in some of our discordant cases and as was reported before (30). Interestingly, similar to the NOPHO group (29) we observed that the concordance was higher in precursor B when compared with T-cell ALL.…”

Section: Discussionsupporting

confidence: 82%

“…Per time point best qualitative agreement was in exchanged LMD from D-15 (86%) as opposed to those from D-33 (52%). Also in the NOPHO QC study (29) at a cutoff level 10, laboratories obtained a high concordance (91.6%). Remarkably, in our study, with no prior standardization and utilizing two very different FCM-MRD methodologies, qualitative agreement was 80% for D-33 and quantitative agreement of D-15 samples was 80.8%.…”

Section: Discussionmentioning

confidence: 85%

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Prospective comparison of two flow cytometry methodologies for monitoring minimal residual disease in a multicenter treatment protocol of childhood acute lymphoblastic leukemia

Luria

Rosenthal

Steinberg

et al. 2010

Cytometry Part B Clinical

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Section: Discussionsupporting

confidence: 82%

Section: Discussionmentioning

confidence: 85%

Prospective comparison of two flow cytometry methodologies for monitoring minimal residual disease in a multicenter treatment protocol of childhood acute lymphoblastic leukemia

Luria

Rosenthal

Steinberg

et al. 2010

Cytometry Part B Clinical

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“…Despite differences in cytometers and software usage, blinded inter-laboratory tests of list-mode data interpretation gave highly concordant results (intraclass correla- robustness of this approach in refining MRD-based stratification with measurements on day 15 (37). The feasibility of standardized multicentric MRD assessment has also been shown by others groups (66,67). Six-eightcolor-FCM MRD techniques are currently employed for leukemia immunophenotyping.…”

Section: Standardization Of Flow Cytometric Methods Formentioning

confidence: 90%

Detection of minimal residual disease in pediatric acute lymphoblastic leukemia

Gaipa

Basso

Biondi

et al. 2013

Cytometry Part B Clinical

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Minimal residual disease (MRD) is a powerful predictor of the overall response to treatment in childhood acute lymphoblastic leukemia (ALL). INTRODUCTIONMost children with acute lymphoblastic leukemia (ALL) achieve complete remission with current treatment regimens but leukemia relapse, the main cause of treatment failure, still occurs in a significant proportion of patients (1). Periodic assessment of treatment response provides an indication of the sensitivity of leukemic cells to chemotherapy and of the overall treatment effectiveness. Historically, treatment response has been monitored by morphological examination of bone marrow aspirates, a task which is a fundamental component of the clinical care of patients with ALL (2). Because this approach has a limited sensitivity and specificity, it can result in failure to detect residual leukemic cells, potentially leading to under-treatment and an increase risk of relapse. Conversely, misclassification of normal cells as ALL blasts may result in over-treatment and an increase in the risk of treatment-related morbidity.Over the last 2-3 decades, much effort has been made to develop accurate and sensitive methods that could determine response to treatment more precisely than morphology, and to detect residual leukemia persisting in patients considered to be in morphologic remission, i.e. minimal residual disease (MRD) (3,4). Many studies have demonstrated that MRD is a powerful predictor of clinical outcome in childhood ALL (5-12), supporting the use of a more stringent definition of hematological remission based on MRD assays rather than morphology (13). METHODOLOGIES FOR MRD DETECTIONTo be informative, MRD assays for ALL should allow to the detection of one leukemic cell among 10,000 normal cells or more. They should also reliably discriminate leukemic and normal cells, and allow a timely output of (14)(15)(16)(17)(18). Currently, the most reliable methods to study MRD in ALL are flow cytometric (FCM) analysis of leukemia-associated immunophenotypes (i.e., aberrant phenotypes expressed in leukemic cells but not in normal bone marrow or peripheral blood cells), and polymerase chain reaction (PCR) amplification of antigen receptor gene rearrangements (2,14-23); gene fusion transcripts can also be used as PCR targets in some cases (24). The main features of these techniques are outlined in Table 1. A BRIEF HISTORY OF THE DEVELOPMENT OF MULTICOLORFLOW CYTOMETRY IMMUNOPHENOTYPING Antigen expression is assessed by quantification of the signal emitted by fluorochrome-conjugated-specific monoclonal antibodies (MoAb). Fluorescein excited by an argon laser was initially used in the Herzenberg laboratory, followed by two-color fluorescence detection (25).Then, additional antibody-conjugated fluorochromes were developed to increase the number of "colors" (26). From the 1980s, the capacity of several molecules to absorb and transfer energy to other fluorescent molecules was exploited to produce tandem dyes such as PETexas Red, PE-Cy5, PE Cy7, and Alexa (27,28), thus many la...

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“…Существен-ными недостатками мониторинга МОБ методом про-точной цитометрии по сравнению с количественной полимеразной цепной реакцией (ПЦР) являются субъективность и сложность стандартизации в рамках многоцентровых исследований [8,14]. В то время как технология молекулярно-генетического ис следования МОБ хорошо отработана и стандартизована [8,14,15], опубликовано лишь несколько работ по начальным этапам стандартизации цитометрического мониторин-га ОЛЛ в рамках отдельных исследовательских групп [16][17][18].…”

Section: фундаментальные исследования в практической медицине на соврunclassified

“…Однако сложности применения данного варианта ПЦР определяют необходимость разработ-ки стандартизованных протоколов определения МОБ проточной цитометрией в рамках различных терапев-тических протоколов. На данный момент такие по-пытки проводятся группами AIEOP-BFM [16], UKALL [17], NOPHO [18]. Кроме того, высокий уровень стан-дартизации определения МОБ при ОЛЛ предлагает не связанная с определенными терапевтическими протоколами группа EuroFlow [14].…”

Section: рис 3 пример последовательного выделения опухолевых клетокunclassified

Standardization of Flow Cytometric Minimal Residual Disease Monitoring in Children With B-Cell Precursor Acute Lymphoblastic Leukemia. Russia–belarus Multicenter Group Experience

Popov¹,

Belevtsev²,

Боякова³

et al. 2016

Onkogematologiâ

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Quality Control of Flow Cytometry Data Analysis for Evaluation of Minimal Residual Disease in Bone Marrow From Acute Leukemia Patients During Treatment

Cited by 22 publications

References 22 publications

Prospective comparison of two flow cytometry methodologies for monitoring minimal residual disease in a multicenter treatment protocol of childhood acute lymphoblastic leukemia

Prospective comparison of two flow cytometry methodologies for monitoring minimal residual disease in a multicenter treatment protocol of childhood acute lymphoblastic leukemia

Detection of minimal residual disease in pediatric acute lymphoblastic leukemia

Standardization of Flow Cytometric Minimal Residual Disease Monitoring in Children With B-Cell Precursor Acute Lymphoblastic Leukemia. Russia–belarus Multicenter Group Experience

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