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51. Interlaboratory Analytical Validation of a Next-Generation Sequencing Strategy for Clonotypic Assessment and Minimal Residual Disease Monitoring in Multiple Myeloma

Author: Medina, Alejandro, primary, Jiménez, Cristina, additional, Puig, Noemí, additional, Sarasquete, María Eugenia, additional, Flores-Montero, Juan, additional, García-Álvarez, María, additional, Prieto-Conde, Isabel, additional, Chillón, Carmen, additional, Alcoceba, Miguel, additional, González-Calle, Verónica, additional, Gutiérrez, Norma C., additional, Jacobsen, Austin, additional, Vigil, Edgar, additional, Hutt, Kasey, additional, Huang, Ying, additional, Orfao, Alberto, additional, González, Marcos, additional, Miller, Jeffrey, additional, and García-Sanz, Ramón, additional
Published: 2021
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52. Reference Values to Assess Hemodilution and Warn of Potential False-Negative Minimal Residual Disease Results in Myeloma

Author: Puig, Noemí, primary, Flores-Montero, Juan, additional, Burgos, Leire, additional, Cedena, María-Teresa, additional, Cordón, Lourdes, additional, Pérez, José-Juan, additional, Sanoja-Flores, Luzalba, additional, Manrique, Irene, additional, Rodríguez-Otero, Paula, additional, Rosiñol, Laura, additional, Martínez-López, Joaquín, additional, Mateos, María-Victoria, additional, Lahuerta, Juan-José, additional, Bladé, Joan, additional, San Miguel, Jesús F., additional, Orfao, Alberto, additional, and Paiva, Bruno, additional
Published: 2021
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53. Minimal Residual Disease in Myeloma: Application for Clinical Care and New Drug Registration

Author: Anderson, Kenneth C., primary, Auclair, Daniel, additional, Adam, Stacey J., additional, Agarwal, Amit, additional, Anderson, Melissa, additional, Avet-Loiseau, Hervé, additional, Bustoros, Mark, additional, Chapman, Jessica, additional, Connors, Dana E., additional, Dash, Ajeeta, additional, Di Bacco, Alessandra, additional, Du, Ling, additional, Facon, Thierry, additional, Flores-Montero, Juan, additional, Gay, Francesca, additional, Ghobrial, Irene M., additional, Gormley, Nicole J., additional, Gupta, Ira, additional, Higley, Howard, additional, Hillengass, Jens, additional, Kanapuru, Bindu, additional, Kazandjian, Dickran, additional, Kelloff, Gary J., additional, Kirsch, Ilan R., additional, Kremer, Brandon, additional, Landgren, Ola, additional, Lightbody, Elizabeth, additional, Lomas, Oliver C., additional, Lonial, Sagar, additional, Mateos, María-Victoria, additional, Montes de Oca, Rocio, additional, Mukundan, Lata, additional, Munshi, Nikhil C., additional, O'Donnell, Elizabeth K., additional, Orfao, Alberto, additional, Paiva, Bruno, additional, Patel, Reshma, additional, Pugh, Trevor J., additional, Ramasamy, Karthik, additional, Ray, Jill, additional, Roshal, Mikhail, additional, Ross, Jeremy A., additional, Sigman, Caroline C., additional, Thoren, Katie L., additional, Trudel, Suzanne, additional, Ulaner, Gary, additional, Valente, Nancy, additional, Weiss, Brendan M., additional, Zamagni, Elena, additional, and Kumar, Shaji K., additional
Published: 2021
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54. Minimal residual disease in Myeloma: Application for clinical care and new drug registration

Author: Anderson, Kenneth, Auclair, Daniel, Adam, Stacey J., Agarwal, Amit, Anderson, Melissa, Avet-Loiseau, Hervé, Bustoros, Mark, Chapman, Jessica, Connors, Dana E., Dash, Ajeeta B., Di Bacco, Alessandra, Du, Ling, Facon, Thierry, Flores-Montero, Juan, Gay, Francesca, Ghobrial, Irene M., Gormley, Nicole J., Gupta, Ira, Higley, Howard, Hillengass, Jens, Kanapuru, Bindu, Kazandjian, Dickran, Kelloff, Gary J., Kirsch, Ilan R., Kremer, Brandon, Landgren, Ola, Lightbody, Elizabeth, Lomas, Oliver C., Lonial, Sagar, Mateos, Maria Victoria, Montes de Oca, Rocío, Mukundan, Lata, Munshi, Nikhil, O’Donnell, Elizabeth K., Orfao, Alberto, Paiva, Bruno, Patel, Reshma, Pugh, Trevor J., Ramasamy, Karthik, Ray, Jill, Roshal, Mikhail, Ross, J. A., Sigman, Caroline C., Thoren, Katie L., Trudel, Suzanne, Ulaner, Gary, Valente, Nancy, Weiss, Brendan M., Zamagni, Elena, and Kumar, S.
Abstract: The development of novel agents has transformed the treatment paradigm for multiple myeloma, with minimal residual disease (MRD) negativity now achievable across the entire disease spectrum. Bone marrow–based technologies to assess MRD, including approaches using next-generation flow and next-generation sequencing, have provided real-time clinical tools for the sensitive detection and monitoring of MRD in patients with multiple myeloma. Complementary liquid biopsy–based assays are now quickly progressing with some, such as mass spectrometry methods, being very close to clinical use, while others utilizing nucleic acid–based technologies are still developing and will prove important to further our understanding of the biology of MRD. On the regulatory front, multiple retrospective individual patient and clinical trial level meta-analyses have already shown and will continue to assess the potential of MRD as a surrogate for patient outcome. Given all this progress, it is not surprising that a number of clinicians are now considering using MRD to inform real-world clinical care of patients across the spectrum from smoldering myeloma to relapsed refractory multiple myeloma, with each disease setting presenting key challenges and questions that will need to be addressed through clinical trials. The pace of advances in targeted and immune therapies in multiple myeloma is unprecedented, and novel MRD-driven biomarker strategies are essential to accelerate innovative clinical trials leading to regulatory approval of novel treatments and continued improvement in patient outcomes.
Published: 2021

55. Reference Values to Assess Hemodilution and Warn of Potential False-Negative Minimal Residual Disease Results in Myeloma

Author: Puig, Noemí, Flores Montero, Juan, Burgos, Leire, Cedena, María Teresa, Cordón, Lourdes, Pérez, José Juan, Sanoja Flores, Luzalba, Manrique, Irene, Rodríguez Otero, Paula, Rosiñol, Laura, Martínez López, Joaquín, Mateos, María Victoria, Lahuerta, Juan José, Bladé, Joan, San Miguel, Jesús F., Orfao, Alberto, Paiva, Bruno, Puig, Noemí, Flores Montero, Juan, Burgos, Leire, Cedena, María Teresa, Cordón, Lourdes, Pérez, José Juan, Sanoja Flores, Luzalba, Manrique, Irene, Rodríguez Otero, Paula, Rosiñol, Laura, Martínez López, Joaquín, Mateos, María Victoria, Lahuerta, Juan José, Bladé, Joan, San Miguel, Jesús F., Orfao, Alberto, and Paiva, Bruno
Abstract: This study was supported by grants from the Centro de Investigación Biomédica en Red—Área de Oncología—del Instituto de Salud Carlos III (CIBERONC; CB16/12/00369, CB16/12/00400, CB16/12/00233 and CB16/12/00284); Instituto de Salud Carlos III/Subdirección General de Investigación Sanitaria and co-financed by FEDER funds (FIS No. PI15/01956, PI15/02049, PI15/02062, PI18/01709, PI18/01673 and PI19/01451); the Cancer Research UK (C355/A26819), FCAECC and AIRC under the Accelerator Award Programme (EDITOR); the Black Swan Research Initiative of the International Myeloma Foundation and the European Research Council (ERC) 2015 Starting Grant (Contract 680200 MYELOMANEXT). This study was supported by the Riney Family Multiple Myeloma Research Program Fund., Background: Whereas, in most patients with multiple myeloma (MM), achieving undetectable MRD anticipates a favorable outcome, some others relapse shortly afterwards. Although one obvious explanation for this inconsistency is the use of nonrepresentative marrow samples due to hemodilution, there is no guidance on how to evaluate this issue. Methods: Since B-cell precursors, mast cells and nucleated red blood cells are normally absent in peripheral blood, we analyzed them in 1404 bone marrow (BM) aspirates obtained in numerous disease settings and in 85 healthy adults (HA). Results: First, we confirmed the systematic detection of the three populations in HA, as well as the nonreduced numbers with aging. Pairwise comparisons between HA and MM patients grouped according to age and treatment showed significant variability, suggesting that hemodilution should be preferably evaluated with references obtained from patients treated with identical regimens. Leveraging the MRD results from 118 patients, we showed that a comparison with HA of similar age could also inform on potential hemodilution. Conclusions: Our study supports the routine assessment of BM cellularity to evaluate hemodilution, since reduced BM-specific cell types as compared to reference values (either treatment-specific or from HA if the former are unavailable) could indicate hemodilution and a false-negative MRD result., Unión Europea, Consejo Europeo de Investigación, Centro de Investigación Biomédica en Red, Instituto de Salud Carlos III, Cancer Research UK, The Italian Foundation for Cancer Research (AIRCE), Fundación Internacional del Mieloma, Asociación Española contra el Cáncer, Depto. de Medicina, Fac. de Medicina, TRUE, pub
Published: 2021

56. Reference Values to Assess Hemodilution and Warn of Potential False-Negative Minimal Residual Disease Results in Myeloma

Author: Centro de Investigación Biomédica en Red Cáncer (España), Instituto de Salud Carlos III, European Commission, Cancer Research UK, Fundación Científica Asociación Española Contra el Cáncer, Associazione Italiana per la Ricerca sul Cancro, International Myeloma Foundation, European Research Council, Paula and Rodger Riney Foundation, Puig, Noemi, Flores-Montero, Juan, Burgos, Leire, Cedena, Maria-Teresa, Cordón, Lourdes, Pérez, José J., Sanoja-Flores, Luzalba, Manrique, Irene, Rodríguez-Otero, Paula, Rosiñol, Laura, Martínez-López, Joaquín, Mateos, Maria Victoria, Lahuerta, Juan José, Bladé, Joan, San Miguel, Jesús F., Orfao, Alberto, Paiva, Bruno, Centro de Investigación Biomédica en Red Cáncer (España), Instituto de Salud Carlos III, European Commission, Cancer Research UK, Fundación Científica Asociación Española Contra el Cáncer, Associazione Italiana per la Ricerca sul Cancro, International Myeloma Foundation, European Research Council, Paula and Rodger Riney Foundation, Puig, Noemi, Flores-Montero, Juan, Burgos, Leire, Cedena, Maria-Teresa, Cordón, Lourdes, Pérez, José J., Sanoja-Flores, Luzalba, Manrique, Irene, Rodríguez-Otero, Paula, Rosiñol, Laura, Martínez-López, Joaquín, Mateos, Maria Victoria, Lahuerta, Juan José, Bladé, Joan, San Miguel, Jesús F., Orfao, Alberto, and Paiva, Bruno
Abstract: [Simple Summary] Although the majority of patients with myeloma who achieve undetectable minimal residual disease show prolonged survival, some of them relapse shortly afterwards. False-negative results due to hemodiluted bone marrow samples could explain this inconsistency, but there is no guidance on how to evaluate them. We analyzed three cell populations normally absent in peripheral blood in 1404 aspirates obtained in numerous disease settings and in 85 healthy adults. Pairwise comparisons according to age and treatment showed significant variability, thus suggesting that hemodilution should be preferably evaluated with references obtained after receiving identical regimens. Leveraging the minimal residual disease results from 118 patients, we showed that a comparison with age-matched healthy adults could also inform on potential hemodilution. Our study supports the routine assessment of bone marrow cellularity to evaluate hemodilution, using as reference values either treatment-specific or from healthy adults if the former are unavailable., [Abstract] Background: Whereas, in most patients with multiple myeloma (MM), achieving undetectable MRD anticipates a favorable outcome, some others relapse shortly afterwards. Although one obvious explanation for this inconsistency is the use of nonrepresentative marrow samples due to hemodilution, there is no guidance on how to evaluate this issue. Methods: Since B-cell precursors, mast cells and nucleated red blood cells are normally absent in peripheral blood, we analyzed them in 1404 bone marrow (BM) aspirates obtained in numerous disease settings and in 85 healthy adults (HA). Results: First, we confirmed the systematic detection of the three populations in HA, as well as the nonreduced numbers with aging. Pairwise comparisons between HA and MM patients grouped according to age and treatment showed significant variability, suggesting that hemodilution should be preferably evaluated with references obtained from patients treated with identical regimens. Leveraging the MRD results from 118 patients, we showed that a comparison with HA of similar age could also inform on potential hemodilution. Conclusions: Our study supports the routine assessment of BM cellularity to evaluate hemodilution, since reduced BM-specific cell types as compared to reference values (either treatment-specific or from HA if the former are unavailable) could indicate hemodilution and a false-negative MRD result.
Published: 2021

57. B-cell regeneration profile and minimal residual disease status in bone marrow of treated multiple myeloma patients

Author: International Myeloma Foundation, European Commission, Centro de Investigación Biomédica en Red Cáncer (España), Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (Brasil), Fundaçao Capes (Brasil), Ministerio de Educación, Cultura y Deporte (España), Fundação Carlos Chagas Filho de Amparo à Pesquisa do Estado do Rio de Janeiro, Conselho Nacional de Desenvolvimento Científico e Tecnológico (Brasil), Mendonça de Pontes, Robéria, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Puig, Noemi, Pessoa de Magalhães, Roberto J., Corral-Mateos, A., Salgado, Anna Beatriz, García-Sánchez, O., Pérez-Morán, José, Mateos, Maria Victoria, Burgos, Leire, Paiva, Bruno, Marvelde, Jeroen G. te, Velden, Vincent H. J. van der, Aguilar, Carlos, Bárez, Abelardo, García-Mateo, Aránzazu, Labrador, Jorge, Leoz, Pilar, Aguilera-Sanz, C., Orfao, Alberto, International Myeloma Foundation, European Commission, Centro de Investigación Biomédica en Red Cáncer (España), Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (Brasil), Fundaçao Capes (Brasil), Ministerio de Educación, Cultura y Deporte (España), Fundação Carlos Chagas Filho de Amparo à Pesquisa do Estado do Rio de Janeiro, Conselho Nacional de Desenvolvimento Científico e Tecnológico (Brasil), Mendonça de Pontes, Robéria, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Puig, Noemi, Pessoa de Magalhães, Roberto J., Corral-Mateos, A., Salgado, Anna Beatriz, García-Sánchez, O., Pérez-Morán, José, Mateos, Maria Victoria, Burgos, Leire, Paiva, Bruno, Marvelde, Jeroen G. te, Velden, Vincent H. J. van der, Aguilar, Carlos, Bárez, Abelardo, García-Mateo, Aránzazu, Labrador, Jorge, Leoz, Pilar, Aguilera-Sanz, C., and Orfao, Alberto
Abstract: B-cell regeneration during therapy has been considered as a strong prognostic factor in multiple myeloma (MM). However, the effects of therapy and hemodilution in bone marrow (BM) B-cell recovery have not been systematically evaluated during follow-up. MM (n = 177) and adult (≥50y) healthy donor (HD; n = 14) BM samples were studied by next-generation flow (NGF) to simultaneously assess measurable residual disease (MRD) and residual normal B-cell populations. BM hemodilution was detected in 41 out of 177 (23%) patient samples, leading to lower total B-cell, B-cell precursor (BCP) and normal plasma cell (nPC) counts. Among MM BM, decreased percentages (vs. HD) of BCP, transitional/naïve B-cell (TBC/NBC) and nPC populations were observed at diagnosis. BM BCP increased after induction therapy, whereas TBC/NBC counts remained abnormally low. At day+100 postautologous stem cell transplantation, a greater increase in BCP with recovered TBC/NBC cell numbers but persistently low memory B-cell and nPC counts were found. At the end of therapy, complete response (CR) BM samples showed higher CD19− nPC counts vs. non-CR specimens. MRD positivity was associated with higher BCP and nPC percentages. Hemodilution showed a negative impact on BM B-cell distribution. Different BM B-cell regeneration profiles are present in MM at diagnosis and after therapy with no significant association with patient outcome.
Published: 2021

58. B-cell regeneration profile and minimal residual disease status in bone marrow of treated multiple myeloma patients

Author: de Pontes, Robéria Mendonça, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Puig, Noemi, Pessoa de Magalhães, Roberto J., Corral-Mateos, Alba, Salgado, Anna Beatriz, García-Sánchez, Omar, Pérez-Morán, José, Mateos, Maria Victoria, Burgos, Leire, Paiva, Bruno, Marvelde, Jeroen Te, van der Velden, Vincent H.J., Aguilar, Carlos, Bárez, Abelardo, García-Mateo, Aranzazú, Labrador, Jorge, Leoz, Pilar, Aguilera-Sanz, Carmen, Durie, Brian, van Dongen, Jacques J.M., Maiolino, Angelo, da Costa, Elaine Sobral, Orfao, Alberto, de Pontes, Robéria Mendonça, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Puig, Noemi, Pessoa de Magalhães, Roberto J., Corral-Mateos, Alba, Salgado, Anna Beatriz, García-Sánchez, Omar, Pérez-Morán, José, Mateos, Maria Victoria, Burgos, Leire, Paiva, Bruno, Marvelde, Jeroen Te, van der Velden, Vincent H.J., Aguilar, Carlos, Bárez, Abelardo, García-Mateo, Aranzazú, Labrador, Jorge, Leoz, Pilar, Aguilera-Sanz, Carmen, Durie, Brian, van Dongen, Jacques J.M., Maiolino, Angelo, da Costa, Elaine Sobral, and Orfao, Alberto
Abstract: B-cell regeneration during therapy has been considered as a strong prognostic factor in multiple myeloma (MM). However, the effects of therapy and hemodilution in bone marrow (BM) B-cell recovery have not been systematically evaluated during follow-up. MM (n = 177) and adult (≥50y) healthy donor (HD; n = 14) BM samples were studied by next-generation flow (NGF) to simultaneously assess measurable residual disease (MRD) and residual normal B-cell populations. BM hemodilution was detected in 41 out of 177 (23%) patient samples, leading to lower total B-cell, B-cell precursor (BCP) and normal plasma cell (nPC) counts. Among MM BM, decreased percentages (vs. HD) of BCP, transitional/naïve B-cell (TBC/NBC) and nPC populations were observed at diagnosis. BM BCP increased after induction therapy, whereas TBC/NBC counts remained abnormally low. At day+100 postautologous stem cell transplantation, a greater increase in BCP with recovered TBC/NBC cell numbers but persistently low memory B-cell and nPC counts were found. At the end of therapy, complete response (CR) BM samples showed higher CD19− nPC counts vs. non-CR specimens. MRD positivity was associated with higher BCP and nPC percentages. Hemodilution showed a negative impact on BM B-cell distribution. Different BM B-cell regeneration profiles are present in MM at diagnosis and after therapy with no significant association with patient outcome.
Published: 2021

59. B-Cell Regeneration Profile and Minimal Residual Disease Status in Bone Marrow of Treated Multiple Myeloma Patients

Author: Mendonça de Pontes, Robéria, primary, Flores-Montero, Juan, additional, Sanoja-Flores, Luzalba, additional, Puig, Noemi, additional, Pessoa de Magalhães, Roberto J., additional, Corral-Mateos, Alba, additional, Salgado, Anna Beatriz, additional, García-Sánchez, Omar, additional, Pérez-Morán, José, additional, Mateos, Maria-Victoria, additional, Burgos, Leire, additional, Paiva, Bruno, additional, te Marvelde, Jeroen, additional, van der Velden, Vincent H. J., additional, Aguilar, Carlos, additional, Bárez, Abelardo, additional, García-Mateo, Aranzazú, additional, Labrador, Jorge, additional, Leoz, Pilar, additional, Aguilera-Sanz, Carmen, additional, Durie, Brian, additional, van Dongen, Jacques J. M., additional, Maiolino, Angelo, additional, Sobral da Costa, Elaine, additional, and Orfao, Alberto, additional
Published: 2021
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60. Measurable Residual Disease by Next-Generation Flow Cytometry in Multiple Myeloma

Author: Celgene, Janssen Biotech, Sanofi, Takeda Pharmaceutical Company, Amgen, Gilead Sciences, Incyte, Bristol-Myers Squibb, Prothena, Pfizer, Paiva, Bruno, Puig, Noemi, Cedena, Maria-Teresa, Rosiñol, Laura, Cordón, Lourdes, Vidriales, Maria Belén, Burgos, Leire, Flores-Montero, Juan, Sanoja-Flores, Luzalba, López-Anglada, Lucía, Maldonado, Roberto, Cruz, Javier de la, Gutiérrez, Norma Carmen, Calasanz, Mª Jose, Martín-Ramos, María-Luisa, García-Sanz, Ramón, Martínez-López, Joaquín, Oriol, Albert, Blanchard, María Jesús, Ríos, Rafael, Martín, Jesús, Martínez-Martínez, Rafael, Sureda, Anna, Hernandez, Miguel T., Rubia, Javier de la, Krsnik, Isabel, Moraleda, José María, Palomera, Luis, Bargay, Joan, Celgene, Janssen Biotech, Sanofi, Takeda Pharmaceutical Company, Amgen, Gilead Sciences, Incyte, Bristol-Myers Squibb, Prothena, Pfizer, Paiva, Bruno, Puig, Noemi, Cedena, Maria-Teresa, Rosiñol, Laura, Cordón, Lourdes, Vidriales, Maria Belén, Burgos, Leire, Flores-Montero, Juan, Sanoja-Flores, Luzalba, López-Anglada, Lucía, Maldonado, Roberto, Cruz, Javier de la, Gutiérrez, Norma Carmen, Calasanz, Mª Jose, Martín-Ramos, María-Luisa, García-Sanz, Ramón, Martínez-López, Joaquín, Oriol, Albert, Blanchard, María Jesús, Ríos, Rafael, Martín, Jesús, Martínez-Martínez, Rafael, Sureda, Anna, Hernandez, Miguel T., Rubia, Javier de la, Krsnik, Isabel, Moraleda, José María, Palomera, Luis, and Bargay, Joan
Abstract: [Purpose] Assessing measurable residual disease (MRD) has become standard with many tumors, but the clinical meaning of MRD in multiple myeloma (MM) remains uncertain, particularly when assessed by next-generation flow (NGF) cytometry. Thus, we aimed to determine the applicability and sensitivity of the flow MRD-negative criterion defined by the International Myeloma Working Group (IMWG)., [Patients and methods] In the PETHEMA/GEM2012MENOS65 trial, 458 patients with newly diagnosed MM had longitudinal assessment of MRD after six induction cycles with bortezomib, lenalidomide, and dexamethasone (VRD), autologous transplantation, and two consolidation courses with VRD. MRD was assessed in 1,100 bone marrow samples from 397 patients; the 61 patients without MRD data discontinued treatment during induction and were considered MRD positive for intent-to-treat analysis. The median limit of detection achieved by NGF was 2.9 × 10−6. Patients received maintenance (lenalidomide ± ixazomib) according to the companion PETHEMA/GEM2014MAIN trial., [Results] Overall, 205 (45%) of 458 patients had undetectable MRD after consolidation, and only 14 of them (7%) have experienced progression thus far; seven of these 14 displayed extraosseous plasmacytomas at diagnosis and/or relapse. Using time-dependent analysis, patients with undetectable MRD had an 82% reduction in the risk of progression or death (hazard ratio, 0.18; 95% CI, 0.11 to 0.30; P < .001) and an 88% reduction in the risk of death (hazard ratio, 0.12; 95% CI, 0.05 to 0.29; P < .001). Timing of undetectable MRD (after induction v intensification) had no impact on patient survival. Attaining undetectable MRD overcame poor prognostic features at diagnosis, including high-risk cytogenetics. By contrast, patients with Revised International Staging System III status and positive MRD had dismal progression-free and overall survivals (median, 14 and 17 months, respectively). Maintenance increased the rate of undetectable MRD by 17%., [Conclusions] The IMWG flow MRD-negative response criterion is highly applicable and sensitive to evaluate treatment efficacy in MM.
Published: 2020

61. Automated identification of leukocyte subsets improves standardization of database-guided expert-supervised diagnostic orientation in acute leukemia: a EuroFlow study

Author: European Commission, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), Agencia Estatal de Investigación (España), Ministerio de Ciencia, Innovación y Universidades (España), Silesian University of Technology, Lhermitte, Ludovic, Barreau, Sylvain, Morf, Daniela, Fernández, Paula, Grigore, Georgiana Emilia, Barrena, Susana, Bie, Maaike de, Flores-Montero, Juan, Brüggemann, Monika, Mejstrikova, Ester, Nierkens, Stefan, Burgos, Leire, Caetano, J., Gaipa, Giuseppe, Buracchi, Chiara, Sobral da Costa, E., Sedek, Lukasz, Szczepanski, Tomasz, Aanei, Carmen-Mariana, Sluijs-Gelling, Alita J. van der, Hernández, Alejandro, Fluxá, Rafael, Lécrevisse, Quentin, Pedreira, C. E., Dongen, J. J. M. van, Orfao, Alberto, Velden, Vincent H. J. van der, European Commission, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), Agencia Estatal de Investigación (España), Ministerio de Ciencia, Innovación y Universidades (España), Silesian University of Technology, Lhermitte, Ludovic, Barreau, Sylvain, Morf, Daniela, Fernández, Paula, Grigore, Georgiana Emilia, Barrena, Susana, Bie, Maaike de, Flores-Montero, Juan, Brüggemann, Monika, Mejstrikova, Ester, Nierkens, Stefan, Burgos, Leire, Caetano, J., Gaipa, Giuseppe, Buracchi, Chiara, Sobral da Costa, E., Sedek, Lukasz, Szczepanski, Tomasz, Aanei, Carmen-Mariana, Sluijs-Gelling, Alita J. van der, Hernández, Alejandro, Fluxá, Rafael, Lécrevisse, Quentin, Pedreira, C. E., Dongen, J. J. M. van, Orfao, Alberto, and Velden, Vincent H. J. van der
Abstract: Precise classification of acute leukemia (AL) is crucial for adequate treatment. EuroFlow has previously designed an AL orientation tube (ALOT) to guide toward the relevant classification panel and final diagnosis. In this study, we designed and validated an algorithm for automated (database-supported) gating and identification (AGI tool) of cell subsets within samples stained with ALOT. A reference database of normal peripheral blood (PB, n = 41) and bone marrow (BM; n = 45) samples analyzed with the ALOT was constructed, and served as a reference for the AGI tool to automatically identify normal cells. Populations not unequivocally identified as normal cells were labeled as checks and were classified by an expert. Additional normal BM (n = 25) and PB (n = 43) and leukemic samples (n = 109), analyzed in parallel by experts and the AGI tool, were used to evaluate the AGI tool. Analysis of normal PB and BM samples showed low percentages of checks (<3% in PB, <10% in BM), with variations between different laboratories. Manual analysis and AGI analysis of normal and leukemic samples showed high levels of correlation between cell numbers (r2 > 0.95 for all cell types in PB and r2 > 0.75 in BM) and resulted in highly concordant classification of leukemic cells by our previously published automated database-guided expert-supervised orientation tool for immunophenotypic diagnosis and classification of acute leukemia (Compass tool). Similar data were obtained using alternative, commercially available tubes, confirming the robustness of the developed tools. The AGI tool represents an innovative step in minimizing human intervention and requirements in expertise, toward a “sample-in and result-out” approach which may result in more objective and reproducible data analysis and diagnostics. The AGI tool may improve quality of immunophenotyping in individual laboratories, since high percentages of checks in normal samples are an alert on the quality of the internal procedures.
Published: 2020

62. Circulating tumor cells for comprehensive and multiregional non-invasive genetic characterization of multiple myeloma

Author: Centro de Investigación Biomédica en Red Cáncer (España), Instituto de Salud Carlos III, Cancer Research UK, Asociación Española Contra el Cáncer, European Commission, Ministerio de Ciencia e Innovación (España), European Research Council, International Myeloma Foundation, Qatar National Research Fund, Leukemia Research Foundation, Multiple Myeloma Research Foundation, Garcés, Juan José, Bretones, Gabriel, Burgos, Leire, Valdes-Mas, Rafael, Puig, Noemi, Cedena, Maria-Teresa, Alignani, Diego, Rodríguez, Idoia, Álvarez Puente, Diana, García Álvarez, Miguel, Goicoechea, Ibai, Rodríguez, Sara, Calasanz, Mª Jose, Agirre, Xavier, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Rodríguez-Otero, Paula, Ríos, Rafael, Martínez-López, Joaquín, Millacoy, Pamela, Palomera, Luis, Orbe, Rafael del, Pérez-Montaña, Albert, Omri, Halima El, Prósper, Felipe, Mateos, Maria Victoria, Rosiñol, Laura, Bladé, Joan, Lahuerta, Juan José, Orfao, Alberto, López-Otín, Carlos, Miguel, Jesus F. San, Paiva, Bruno, Centro de Investigación Biomédica en Red Cáncer (España), Instituto de Salud Carlos III, Cancer Research UK, Asociación Española Contra el Cáncer, European Commission, Ministerio de Ciencia e Innovación (España), European Research Council, International Myeloma Foundation, Qatar National Research Fund, Leukemia Research Foundation, Multiple Myeloma Research Foundation, Garcés, Juan José, Bretones, Gabriel, Burgos, Leire, Valdes-Mas, Rafael, Puig, Noemi, Cedena, Maria-Teresa, Alignani, Diego, Rodríguez, Idoia, Álvarez Puente, Diana, García Álvarez, Miguel, Goicoechea, Ibai, Rodríguez, Sara, Calasanz, Mª Jose, Agirre, Xavier, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Rodríguez-Otero, Paula, Ríos, Rafael, Martínez-López, Joaquín, Millacoy, Pamela, Palomera, Luis, Orbe, Rafael del, Pérez-Montaña, Albert, Omri, Halima El, Prósper, Felipe, Mateos, Maria Victoria, Rosiñol, Laura, Bladé, Joan, Lahuerta, Juan José, Orfao, Alberto, López-Otín, Carlos, Miguel, Jesus F. San, and Paiva, Bruno
Abstract: Multiple myeloma (MM) patients undergo repetitive bone marrow (BM) aspirates for genetic characterization. Circulating tumor cells (CTCs) are detectable in peripheral blood (PB) of virtually all MM cases and are prognostic, but their applicability for noninvasive screening has been poorly investigated. Here, we used next-generation flow (NGF) cytometry to isolate matched CTCs and BM tumor cells from 53 patients and compared their genetic profile. In eight cases, tumor cells from extramedullary (EM) plasmacytomas were also sorted and whole-exome sequencing was performed in the three spatially distributed tumor samples. CTCs were detectable by NGF in the PB of all patients with MM. Based on the cancer cell fraction of clonal and subclonal mutations, we found that ~22% of CTCs egressed from a BM (or EM) site distant from the matched BM aspirate. Concordance between BM tumor cells and CTCs was high for chromosome arm-level copy number alterations (≥95%) though not for translocations (39%). All high-risk genetic abnormalities except one t(4;14) were detected in CTCs whenever present in BM tumor cells. Noteworthy, ≥82% mutations present in BM and EM clones were detectable in CTCs. Altogether, these results support CTCs for noninvasive risk-stratification of MM patients based on their numbers and genetic profile.
Published: 2020

63. Detection of circulating tumor plasma cells in monoclonal gammopathies: Methods, pathogenic role, and clinical implications

Author: Multiple Myeloma Research Foundation, Sanoja-Flores, Luzalba, Flores-Montero, Juan, Pérez-Andrés, Martin, Puig, Noemi, Orfao, Alberto, Multiple Myeloma Research Foundation, Sanoja-Flores, Luzalba, Flores-Montero, Juan, Pérez-Andrés, Martin, Puig, Noemi, and Orfao, Alberto
Abstract: Cancer dissemination and distant metastasis most frequently require the release of tumor cells into the blood circulation, both in solid tumors and most hematological malignancies, including plasma cell neoplasms. However, detection of blood circulating tumor cells in solid tumors and some hematological malignancies, such as the majority of mature/peripheral B-cell lymphomas and monoclonal gammopathies, has long been a challenge due to their very low frequency. In recent years, the availability of highly-sensitive and standardized methods for the detection of circulating tumor plasma cells (CTPC) in monoclonal gammopathies, e.g., next-generation flow cytometry (NGF), demonstrated the systematic presence of CTPC in blood in virtually every smoldering (SMM) and symptomatic multiple myeloma (MM) patient studied at diagnosis, and in the majority of patients with newly-diagnosed monoclonal gammopathies of undetermined significance (MGUS). These methods set the basis for further detailed characterization of CTPC vs. their bone marrow counterpart in monoclonal gammopathies, to investigate their role in the biology of the disease, and to confirm their strong impact on patient outcome when measured both at diagnosis and after initiating therapy. Here, we review the currently available techniques for the detection of CTPC, and determine their biological features, physiopathological role and clinical significance in patients diagnosed with distinct diagnostic categories of plasma cell neoplasms.
Published: 2020

64. Monocyte Subsets and Serum Inflammatory and Bone-Associated Markers in Monoclonal Gammopathy of Undetermined Significance and Multiple Myeloma

Author: Damasceno, Daniela, primary, Almeida, Julia, additional, Teodosio, Cristina, additional, Sanoja-Flores, Luzalba, additional, Mayado, Andrea, additional, Pérez-Pons, Alba, additional, Puig, Noemi, additional, Arana, Paula, additional, Paiva, Bruno, additional, Solano, Fernando, additional, Romero, Alfonso, additional, Matarraz, Sergio, additional, van den Bossche, Wouter B. L., additional, Flores-Montero, Juan, additional, Durie, Brian, additional, van Dongen, Jacques J. M., additional, and Orfao, Alberto, additional
Published: 2021
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65. Flow Cytometric Immunophenotyping as Diagnostic Tool of Hematopoietic Malignancies

Author: Sędek, Łukasz, primary, Flores-Montero, Juan, additional, Bulsa, Joanna, additional, Barrena, Susana, additional, Almeida, Julia, additional, Orfao, Alberto, additional, and Szczepański, Tomasz, additional
Published: 2012
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66. Flow cytometric minimal residual disease assessment in B‐cell precursor acute lymphoblastic leukaemia patients treated with CD19‐targeted therapies — a EuroFlow study.

Author: Verbeek, Martijn W. C., Buracchi, Chiara, Laqua, Anna, Nierkens, Stefan, Sedek, Lukasz, Flores‐Montero, Juan, Hofmans, Mattias, Sobral de Costa, Elaine, Nováková, Michaela, Mejstrikova, Ester, Barrena, Susana, Kohlscheen, Saskia, Szczepanowski, Monika, Kulis, Jan, Oliveira, Elen, Jugooa, Romana, de Jong, Anja X., Szczepanski, Tomasz, Philippé, Jan, and van Dongen, Jacques J. M.
Subjects: LYMPHOBLASTIC leukemia, ACUTE leukemia, CD19 antigen
Abstract: Summary: The standardized EuroFlow protocol, including CD19 as primary B‐cell marker, enables highly sensitive and reliable minimal residual disease (MRD) assessment in B‐cell precursor acute lymphoblastic leukaemia (BCP‐ALL) patients treated with chemotherapy. We developed and validated an alternative gating strategy allowing reliable MRD analysis in BCP‐ALL patients treated with CD19‐targeting therapies. Concordant data were obtained in 92% of targeted therapy patients who remained CD19‐positive, whereas this was 81% in patients that became (partially) CD19‐negative. Nevertheless, in both groups median MRD values showed excellent correlation with the original MRD data, indicating that, despite higher interlaboratory variation, the overall MRD analysis was correct. [ABSTRACT FROM AUTHOR]
Published: 2022
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67. Blood monitoring of circulating tumor plasma cells by next generation flow in multiple myeloma after therapy

Author: Sanoja-Flores, Luzalba, Flores-Montero, Juan, Puig, Noemi, Contreras-Sanfeliciano, Teresa, Pontes, Roberia, Corral-Mateos, Alba, García-Sánchez, Omar, Díez-Campelo, María, Pessoa de Magalhães, Roberto José, García-Martín, Luis, Alonso-Alonso, José María, García-Mateo, Aranzazú, Aguilar-Franco, Carlos, Labrador, Jorge, Barez-García, Abelardo, Maiolino, Angelo, Paiva, Bruno, San Miguel, Jesús, Sobral da Costa, Elaine, González, Marcos, Mateos, María Victoria, Durie, Brian, van Dongen, Jacques J.M., and Orfao, Alberto
Published: 2019
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68. Comments on EuroFlow standard operating procedures for instrument setup and compensation for BD FACS Canto II, Navios and BD FACS Lyric instruments

Author: Glier, Hana, Novakova, Michaela, te Marvelde, Jeroen, Bijkerk, Andre, Morf, Daniela, Thurner, Daniel, Rejlova, Katerina, Lange, Sandra, Finke, Judith, van der Sluijs-Gelling, Alita, Sedek, Lukasz, Flores-Montero, Juan, Böttcher, Sebastian, Fernandez, Paula, Ritgen, Matthias, van Dongen, Jacques J.M., Orfao, Alberto, van der Velden, Vincent H.J., and Kalina, Tomas
Published: 2019
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69. Frequent issues and lessons learned from EuroFlow QA

Author: Kalina, Tomas, Brdickova, Nadezda, Glier, Hana, Fernandez, Paula, Bitter, Marieke, Flores-Montero, Juan, van Dongen, Jacques J.M., and Orfao, Alberto
Published: 2019
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70. STAT3 and STAT5B Mutations in T/NK-Cell Chronic Lymphoproliferative Disorders of Large Granular Lymphocytes (LGL): Association with Disease Features

Author: Muñoz-García, Noemí, primary, Jara-Acevedo, María, additional, Caldas, Carolina, additional, Bárcena, Paloma, additional, López, Antonio, additional, Puig, Noemí, additional, Alcoceba, Miguel, additional, Fernández, Paula, additional, Villamor, Neus, additional, Flores-Montero, Juan A., additional, Gómez, Karoll, additional, Lemes, María Angelina, additional, Hernández, Jose Carlos, additional, Álvarez-Twose, Iván, additional, Guerra, Jose Luis, additional, González, Marcos, additional, Orfao, Alberto, additional, and Almeida, Julia, additional
Published: 2020
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71. Detection of Circulating Tumor Plasma Cells in Monoclonal Gammopathies: Methods, Pathogenic Role, and Clinical Implications

Author: Sanoja-Flores, Luzalba, primary, Flores-Montero, Juan, additional, Pérez-Andrés, Martín, additional, Puig, Noemí, additional, and Orfao, Alberto, additional
Published: 2020
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72. How to make usage of the standardized EuroFlow 8-color protocols possible for instruments of different manufacturers

Author: Ministry of Health of the Czech Republic, Ministry of Education, Youth and Sports (Czech Republic), European Commission, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), Novákova, Michaela, Glier, Hana, Brdickova, Nadezda, Vlkova, Marcela, Santos, Ana Helena, Lima, Margarida, Roussel, Mikael, Flores-Montero, Juan, Szczepanski, Tomasz, Velden, Vincent H. J. van der, Fernandez, Paula, Mejstrikova, Ester, Burgos, Leire, Paiva, Bruno, Dongen, J. J. M. van, Orfao, Alberto, Kalina, Tomas, Ministry of Health of the Czech Republic, Ministry of Education, Youth and Sports (Czech Republic), European Commission, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), Novákova, Michaela, Glier, Hana, Brdickova, Nadezda, Vlkova, Marcela, Santos, Ana Helena, Lima, Margarida, Roussel, Mikael, Flores-Montero, Juan, Szczepanski, Tomasz, Velden, Vincent H. J. van der, Fernandez, Paula, Mejstrikova, Ester, Burgos, Leire, Paiva, Bruno, Dongen, J. J. M. van, Orfao, Alberto, and Kalina, Tomas
Abstract: A critical component of the EuroFlow standardization of leukemia/lymphoma immunophenotyping is instrument setup. Initially, the EuroFlow consortium developed a step-by-step standard operating protocol for instrument setup of ≥ 8-color flow cytometers that were available in 2006, when the EuroFlow activities started. Currently, there are 14 instruments from 9 manufacturers capable of 3-laser excitation and ≥ 8 color measurements. The specific adaptations required in the instrument set-up to enable them to acquire the standardized 8-color EuroFlow protocols are described here. Overall, all 14 instruments can be fitted with similar violet, blue and red lasers for simultaneous measurements of ≥ 8 fluorescent dyes. Since individual instruments differ both on their dynamic range (scale) and emission filters, it is not accurate to simply recalculate the target values to different scale, but adjustment of PMT voltages to a given emission filter and fluorochrome, is essential. For this purpose, EuroFlow has developed an approach using Type IIB (spectrally matching) particles to set-up standardized and fully comparable fluorescence measurements, in instruments from different manufacturers, as demonstrated here for the FACSCanto II, and Navios and MACSQuant flow cytometers. Data acquired after such adjustment on any of the tested cytometry platforms could be fully superimposed and therefore analyzed together. The proposed approach can be used to derive target values for any combination of spectrally distinct fluorochromes and any distinct emission filter of any new flow cytometry platform, which enables the measurement of the 8-color EuroFlow panels in a standardized way, by creating superimposable datafiles.
Published: 2019

73. Frequent issues and lessons learned from EuroFlow QA

Author: European Commission, Ministry of Health of the Czech Republic, Ministry of Education, Youth and Sports (Czech Republic), Kalina, Tomas, Brdickova, Nadezda, Glier, Hana, Fernandez, Paula, Bitter, Marieke, Flores-Montero, Juan, Dongen, J. J. M. van, Orfao, Alberto, European Commission, Ministry of Health of the Czech Republic, Ministry of Education, Youth and Sports (Czech Republic), Kalina, Tomas, Brdickova, Nadezda, Glier, Hana, Fernandez, Paula, Bitter, Marieke, Flores-Montero, Juan, Dongen, J. J. M. van, and Orfao, Alberto
Abstract: EuroFlow Quality Assessment was designed to provide a feedback on the quality of the standardization effort in executing the EuroFlow protocols for sample preparation and instrument setup. It was first beta-tested by the members of the EuroFlow consortium internally (2010−2013) and opened to the external participants from 2015 onwards. The goal of participation in the EuroFlow QA is to evaluate whether the technical quality of the data generated by the laboratory is comparable to the data of the EuroFlow members and thus if a non-EuroFlow member participant can use the EuroFlow reference sample database for his own patient evaluation. Also it assesses whether data are sufficiently standardized for automated population gating and alarm notification. By spring 2018, a total 87 laboratories from 32 countries on five continents have registered for the EuroFlow QA program. We evaluated 163 results of 2015–2016 QA rounds, where we noted clear improvement in the score of first-time participants (median score of 91% correct) when they participated second time or later (median score of 94% correct, p = 0,017), which was comparable to EuroFlow member scores (median score of 97% correct). Among frequent mistakes, we found non-adherence to the EuroFlow protocols (improper reagent used), improper gating and some compensation issues. In summary, we show that EuroFlow QA has a positive impact on improvement of standardized data quality of non-member laboratories adhering to the EuroFlow standard operating procedures and reagent panels.
Published: 2019

74. Optimization and testing of dried antibody tube: The EuroFlow LST and PIDOT tubes as examples

Author: Velden, Vincent H. J. van der, Flores-Montero, Juan, Pérez-Andrés, Martin, Martín-Ayuso, Marta, Crespo, Oliver, Blanco, Elena, Kalina, Tomas, Philippé, J., Bonroy, C., Bie, Maaike de, Marvelde, Jeroen G. te, Teodosio, Cristina, Corral-Mateos, A., Kanderová, Veronika, Burg, Mirjam van der, Van Hoof, Dennis, Dongen, J. J. M. van, Velden, Vincent H. J. van der, Flores-Montero, Juan, Pérez-Andrés, Martin, Martín-Ayuso, Marta, Crespo, Oliver, Blanco, Elena, Kalina, Tomas, Philippé, J., Bonroy, C., Bie, Maaike de, Marvelde, Jeroen G. te, Teodosio, Cristina, Corral-Mateos, A., Kanderová, Veronika, Burg, Mirjam van der, Van Hoof, Dennis, and Dongen, J. J. M. van
Abstract: Within EuroFlow, we recently developed screening tubes for hematological malignancies and immune deficiencies. Pipetting of antibodies for such 8-color 12-marker tubes however is time-consuming and prone to operational mistakes. We therefore evaluated dried formats of the lymphocytosis screening tube (LST) and of the primary immune deficiency orientation tube (PIDOT). Both tubes were evaluated on normal and/or on patient samples, comparing the mean fluorescence intensity of specific lymphocyte populations. Our data show that the dried tubes and liquid counterparts give highly comparable staining results, particularly when analyzed in multidimensional plots. In addition, the use of dried tubes may result in a reduced staining variability between different samples and thereby contributes to the generation of more robust data. Therefore, by using ready-to-use reagents in a dried single test tube format, the laboratory efficiency and quality will be improved.
Published: 2019

75. Comments on EuroFlow standard operating procedures for instrument setup and compensation for BD FACS Canto II, Navios and BD FACS Lyric instruments

Author: Ministry of Health of the Czech Republic, Ministry of Education, Youth and Sports (Czech Republic), Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Glier, Hana, Novákova, Michaela, Marvelde, Jeroen G. te, Bijkerk, Andre, Morf, Daniela, Thurner, Daniel, Rejlova, Katerina, Lange, Sandra, Finke, Judith, Sluijs-Gelling, Alita J. van der, Sedek, Lukasz, Flores-Montero, Juan, Böttcher, Sebastian, Fernandez, Paula, Ritgen, Matthias, Dongen, J. J. M. van, Orfao, Alberto, Velden, Vincent H. J. van der, Kalina, Tomas, Ministry of Health of the Czech Republic, Ministry of Education, Youth and Sports (Czech Republic), Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Glier, Hana, Novákova, Michaela, Marvelde, Jeroen G. te, Bijkerk, Andre, Morf, Daniela, Thurner, Daniel, Rejlova, Katerina, Lange, Sandra, Finke, Judith, Sluijs-Gelling, Alita J. van der, Sedek, Lukasz, Flores-Montero, Juan, Böttcher, Sebastian, Fernandez, Paula, Ritgen, Matthias, Dongen, J. J. M. van, Orfao, Alberto, Velden, Vincent H. J. van der, and Kalina, Tomas
Abstract: This commentary discusses particularities of application of the EuroFlow standardization of flow cytometric analyses on three different flow cytometers. The EuroFlow consortium developed a fully standardized approach for flow cytometric immunophenotyping of hematological malignancies and primary immunodeficiencies. Standardized instrument setup is an essential part of EuroFlow standardization. Initially, the EuroFlow Consortium developed and optimized a step-by-step standard operating procedure (SOP) to setup 8-color BD FACSCanto II flow cytometer (Canto), with the later inclusion of Navios (Beckman Coulter) and BD FACSLyric (Lyric). Those SOPs were developed to enable standardized and fully comparable fluorescence measurements in the three flow cytometers. In Canto and Navios, mean fluorescence intensity (MFI) of a reference peak of Rainbow beads calibration particles is used to set up photomultiplier (PMT) voltages for each detector channel in individual instruments to reach the same MFI across distinct instruments. In turn, a new feature of Lyric instruments allows to share collection of attributes that are used to place the positive population at the same position among instruments in the form of assays, as one of its components integrated in the Cytometer Setup and Tracking (CS&T) module. The EuroFlow Lyric assays thus allow for standardized acquisition of 8-color EuroFlow panels on Lyric without the need to setup the PMT voltages on the individual instruments manually. In summary, the standardized instrument setup developed by EuroFlow enables cross-platform inter- and intra-laboratory standardization of flow cytometric measurements. This commentary provides a perspective on the modifications of the standardized EuroFlow instrument setup of Canto, Navios and Lyric instruments that are described in detail in individual instrument-specfic SOPs available at the EuroFlow website.
Published: 2019

76. EuroFlow Lymphoid Screening Tube (LST) data base for automated identification of blood lymphocyte subsets

Author: Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Flores-Montero, Juan, Grigore, Georgiana Emilia, Fluxá, Rafael, Hernández, Juan, Fernandez, Paula, Almeida, Julia, Muñoz, Noemí, Böttcher, Sebastian, Sedek, Lukasz, Velden, Vincent H. J. van der, Barrena, Susana, Hernández, Alejandro, Paiva, Bruno, Lécrevisse, Quentin, Lima, Margarida, Santos, Ana Helena, Dongen, J. J. M. van, Orfao, Alberto, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Flores-Montero, Juan, Grigore, Georgiana Emilia, Fluxá, Rafael, Hernández, Juan, Fernandez, Paula, Almeida, Julia, Muñoz, Noemí, Böttcher, Sebastian, Sedek, Lukasz, Velden, Vincent H. J. van der, Barrena, Susana, Hernández, Alejandro, Paiva, Bruno, Lécrevisse, Quentin, Lima, Margarida, Santos, Ana Helena, Dongen, J. J. M. van, and Orfao, Alberto
Abstract: In recent years the volume and complexity of flow cytometry data has increased substantially. This has led to a greater number of identifiable cell populations in a single measurement. Consequently, new gating strategies and new approaches for cell population definition are required. Here we describe how the EuroFlow Lymphoid Screening Tube (LST) reference data base for peripheral blood (PB) samples was designed, constructed and validated for automated gating of the distinct lymphoid (and myeloid) subsets in PB of patients with chronic lymphoproliferative disorders (CLPD). A total of 46 healthy/reactive PB samples which fulfilled pre-defined technical requirements, were used to construct the LST-PB reference data base. In addition, another set of 92 PB samples (corresponding to 10 healthy subjects, 51 B-cell CLPD and 31 T/NK-cell CLPD patients), were used to validate the automated gating and cell-population labeling tools with the Infinicyt software. An overall high performance of the LST-PB data base was observed with a median percentage of alarmed cellular events of 0.8% in 10 healthy donor samples and of 44.4% in CLPD data files containing 49.8% (range: 1.3–96%) tumor cells. The higher percent of alarmed cellular events in every CLPD sample was due to aberrant phenotypes (75.6% cases) and/or to abnormally increased cell counts (86.6% samples). All 18 (22%) data files that only displayed numerical alterations, corresponded to T/NK-cell CLPD cases which showed a lower incidence of aberrant phenotypes (41%) vs B-cell CLPD cases (100%). Comparison between automated vs expert-bases manual classification of normal (r2 = 0.96) and tumor cell populations (rho = 0.99) showed a high degree of correlation. In summary, our results show that automated gating of cell populations based on the EuroFlow LST-PB data base provides an innovative, reliable and reproducible tool for fast and simplified identification of normal vs pathological B and T/NK lymphocytes in PB of CLPD patie
Published: 2019

77. Fluorochrome choices for multi-color flow cytometry

Author: Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Flores-Montero, Juan, Kalina, Tomas, Corral-Mateos, A., Sanoja-Flores, Luzalba, Pérez-Andrés, Martin, Martín-Ayuso, Marta, Sedek, Lukasz, Rejlova, Katerina, Mayado, Andrea, Fernandez, Paula, Velden, Vincent H. J. van der, Böttcher, Sebastian, Dongen, J. J. M. van, Orfao, Alberto, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Flores-Montero, Juan, Kalina, Tomas, Corral-Mateos, A., Sanoja-Flores, Luzalba, Pérez-Andrés, Martin, Martín-Ayuso, Marta, Sedek, Lukasz, Rejlova, Katerina, Mayado, Andrea, Fernandez, Paula, Velden, Vincent H. J. van der, Böttcher, Sebastian, Dongen, J. J. M. van, and Orfao, Alberto
Abstract: Fluorochrome selection is a key step in designing multi-color antibody panels. The list of available fluorochromes is continuously growing, fitting current needs in clinical flow cytometry to simultaneously use more markers to better define multiple leukocyte subpopulations in a single tube. Several criteria guide fluorochrome selection: i) the fluorescence profiles (excitation and emission), ii) relative brightness, iii) fluorescence overlap, iv) fluorochrome stability, and v) reproducible conjugation to antibodies. Here we used 75 samples (45 bone marrow and 30 blood) to illustrate EuroFlow strategies for evaluation of compatible fluorochromes, and how the results obtained guide fluorochrome selection as a critical step in the antibody-panel building process. Our results allowed identification of optimal fluorescence profiles (e.g. higher fluorescence intensity and/or resolution with limited fluorescence overlap into neighbor channels) for brilliant violet (BV)421 and BV510 in the violet laser and allophycocyanin (APC) hilite 7 (H7) or APC C750 in the red laser vs. other candidate fluorochromes generally applied for the same detectors and here evaluated. Moreover, evaluation of the same characteristics for another group of fluorochromes (e.g. BV605, BV650, PE CF594, AF700 or APC AF700) guided selection of the most appropriate fluorochrome conjugates to be combined in a multi-color antibody panel. Albeit this is a demanding approach, it could be successfully applied for selection of fluorochrome combinations for the EuroFlow antibody panels for diagnosis, classification and monitoring of hematological malignancies and primary immunodeficiencies. Consequently, sets of 8-, 10- and 12-color fluorochrome combinations are proposed as frame of reference for initial antibody panel design.
Published: 2019

78. Circulating Tumor Cells (CTCs) for Comprehensive and Multiregional Non-Invasive Genetic Characterization of Multiple Myeloma (MM)

Author: Garcés, Juan José, primary, Bretones, Gabriel, additional, Burgos, Leire, additional, Valdes-Mas, Rafael, additional, Alignani, Diego, additional, Álvarez Puente, Diana, additional, Goicoechea, Ibai, additional, García Álvarez, Miguel, additional, Garate, Sonia, additional, Rodriguez, Idoia, additional, Calasanz, Maria Jose, additional, Rodriguez, Paula, additional, Rios, Rafael, additional, Martinez-Lopez, Joaquin, additional, Millacoy, Pamela, additional, Palomera, Luis, additional, Del Orbe, Rafael, additional, Pérez, Albert, additional, Agirre, Xabier, additional, Flores-Montero, Juan, additional, Sanoja-Flores, Luzalba, additional, Orfao, Alberto, additional, El Omri, Halima, additional, Prosper, Felipe, additional, Lopez-Otin, Carlos, additional, San-Miguel, Jesús, additional, and Paiva, Bruno, additional
Published: 2019
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79. Transcriptional profiling of circulating tumor cells in multiple myeloma: a new model to understand disease dissemination

Author: Garcés, Juan-Jose, primary, Simicek, Michal, additional, Vicari, Marco, additional, Brozova, Lucie, additional, Burgos, Leire, additional, Bezdekova, Renata, additional, Alignani, Diego, additional, Calasanz, Maria-Jose, additional, Growkova, Katerina, additional, Goicoechea, Ibai, additional, Agirre, Xabier, additional, Pour, Ludek, additional, Prosper, Felipe, additional, Rios, Rafael, additional, Martinez-Lopez, Joaquin, additional, Millacoy, Pamela, additional, Palomera, Luis, additional, Del Orbe, Rafael, additional, Perez-Montaña, Albert, additional, Garate, Sonia, additional, Blanco, Laura, additional, Lasa, Marta, additional, Maiso, Patricia, additional, Flores-Montero, Juan, additional, Sanoja-Flores, Luzalba, additional, Chyra, Zuzana, additional, Vdovin, Alexander, additional, Sevcikova, Tereza, additional, Jelinek, Tomas, additional, Botta, Cirino, additional, El Omri, Halima, additional, Keats, Jonathan, additional, Orfao, Alberto, additional, Hajek, Roman, additional, San-Miguel, Jesus F., additional, and Paiva, Bruno, additional
Published: 2019
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80. Prognostic implications of MRD assessment in multiple myeloma patients: comparison of Next-Generation Sequencing and Next-Generation Flow

Author: Medina, Alejandro, primary, Jiménez, Cristina, additional, Puig, Noemi, additional, Flores-Montero, Juan, additional, Paiva, Bruno, additional, Sarasquete, M Eugenia, additional, Prieto-Conde, Isabel, additional, Garcia-Alvarez, Maria, additional, Chillon, Carmen, additional, Alcoceba, Miguel, additional, Gonzalez-Calle, Veronica, additional, Gutierrez, Norma C., additional, de Arriba, Felipe, additional, Hernandez, Miguel T., additional, Blade, Joan, additional, Martinez-Lopez, Joaquin, additional, Calasanz, Maria-Jose, additional, Lahuerta, Juan-Jose, additional, Mateos, Maria-Victoria, additional, San-Miguel, Jesus, additional, Gonzalez, Marcos, additional, and Garcia-Sanz, Ramon, additional
Published: 2019
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81. Next generation flow for minimally-invasive blood characterization of MGUS and multiple myeloma at diagnosis based on circulating tumor plasma cells (CTPC)

Author: International Myeloma Foundation, Centro de Investigación Biomédica en Red Cáncer (España), Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Junta de Castilla y León, Qatar National Research Fund, Fundación BBVA, European Research Council, Sanoja-Flores, Luzalba, Flores-Montero, Juan, Garcés, Juan José, Paiva, Bruno, Puig, Noemi, García-Mateo, Aránzazu, García-Sánchez, O., Corral-Mateos, A., Burgos, Leire, Blanco, Elena, Hernández-Martín, J., Pontes, R., Díez-Campelo, María, Millacoy, Pamela, Rodríguez-Otero, Paula, Prósper, Felipe, Merino, Jaime, Vidriales, Maria Belén, García-Sanz, Ramón, Romero, Alfonso, Palomera, Luis, Ríos-Tamayo, R., Pérez-Andrés, Martin, Blanco, Juan F., González, Marcos, Dongen, J. J. M. van, Durie, B., Mateos, Maria Victoria, San-Miguel, Jesús, Orfao, Alberto, International Myeloma Foundation, Centro de Investigación Biomédica en Red Cáncer (España), Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Junta de Castilla y León, Qatar National Research Fund, Fundación BBVA, European Research Council, Sanoja-Flores, Luzalba, Flores-Montero, Juan, Garcés, Juan José, Paiva, Bruno, Puig, Noemi, García-Mateo, Aránzazu, García-Sánchez, O., Corral-Mateos, A., Burgos, Leire, Blanco, Elena, Hernández-Martín, J., Pontes, R., Díez-Campelo, María, Millacoy, Pamela, Rodríguez-Otero, Paula, Prósper, Felipe, Merino, Jaime, Vidriales, Maria Belén, García-Sanz, Ramón, Romero, Alfonso, Palomera, Luis, Ríos-Tamayo, R., Pérez-Andrés, Martin, Blanco, Juan F., González, Marcos, Dongen, J. J. M. van, Durie, B., Mateos, Maria Victoria, San-Miguel, Jesús, and Orfao, Alberto
Abstract: Here, we investigated for the first time the frequency and number of circulating tumor plasma cells (CTPC) in peripheral blood (PB) of newly diagnosed patients with localized and systemic plasma cell neoplasms (PCN) using next-generation flow cytometry (NGF) and correlated our findings with the distinct diagnostic and prognostic categories of the disease. Overall, 508 samples from 264 newly diagnosed PCN patients, were studied. CTPC were detected in PB of all active multiple myeloma (MM; 100%), and smoldering MM (SMM) patients (100%), and in more than half (59%) monoclonal gammopathy of undetermined significance (MGUS) cases (p <0.0001); in contrast, CTPC were present in a small fraction of solitary plasmacytoma patients (18%). Higher numbers of CTPC in PB were associated with higher levels of BM infiltration and more adverse prognostic features, together with shorter time to progression from MGUS to MM (p <0.0001) and a shorter survival in MM patients with active disease requiring treatment (p ≤ 0.03). In summary, the presence of CTPC in PB as assessed by NGF at diagnosis, emerges as a hallmark of disseminated PCN, higher numbers of PB CTPC being strongly associated with a malignant disease behavior and a poorer outcome of both MGUS and MM.
Published: 2018

82. Measurable Residual Disease by Next-Generation Flow Cytometry in Multiple Myeloma.

Author: Paiva, Bruno, Puig, Noemi, Cedena, Maria-Teresa, Rosiñol, Laura, Cordón, Lourdes, Vidriales, María-Belén, Burgos, Leire, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Lopez-Anglada, Lucia, Maldonado, Roberto, de la Cruz, Javier, Gutierrez, Norma C., Calasanz, Maria-Jose, Martin-Ramos, Maria-Luisa, Garcia-Sanz, Ramón, Martinez-Lopez, Joaquin, Oriol, Albert, Blanchard, María-Jesús, and Rios, Rafael
Published: 2020
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83. Impact of Treatment on B-Cell Regeneration By Next Generation Flow Cytometry in Patients with Multiple Myeloma

Author: Pontes, Robéria, primary, Flores-Montero, Juan, additional, Sanoja-Flores, Luzalba, additional, Puig, Noemi, additional, Magalhães, Roberto José Pessoa, additional, Mateos, Alba Corral, additional, Salgado, Anna Beatriz, additional, Maiolino, Angelo, additional, Mateos, Maria-Victoria, additional, Paiva, Bruno, additional, da Costa, Elaine Sobral, additional, van Dongen, Jacques JM, additional, and Orfao, Alberto, additional
Published: 2018
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84. Clinical Significance and Transcriptional Profiling of Persistent Minimal Residual Disease (MRD) in Multiple Myeloma (MM) Patients with Standard-Risk (SR) and High-Risk (HR) Cytogenetics

Author: Goicoechea, Ibai, primary, Puig, Noemi, additional, Cedena, María Teresa, additional, Cordon, Lourdes, additional, Vidriales, Maria-Belen, additional, Burgos, Leire, additional, Flores-Montero, Juan, additional, Gutierrez, Norma C., additional, Calasanz, Maria Jose, additional, Martin-Ramos, Maria Luisa, additional, Lara-Astiaso, David, additional, Vilas-Zornoza, Amaia, additional, Alignani, Diego, additional, Rodriguez, Idoia, additional, Sarvide, Sarai, additional, Garcia-Sanz, Ramon, additional, Martinez-Lopez, Joaquin, additional, Oriol, Albert, additional, Rios, Rafael, additional, Martín, Jesús, additional, Martínez, Rafael, additional, Sarra, Josep, additional, Hernández, Miguel T, additional, De La Rubia, Javier, additional, Krsnik, Isabel, additional, Moraleda, Jose Maria, additional, Palomera, Luis, additional, Bargay, Joan, additional, Orfao, Alberto, additional, Rosiñol, Laura, additional, Mateos, Maria-Victoria, additional, Lahuerta, Juan Jose, additional, Bladé, Joan, additional, San-Miguel, Jesus F, additional, and Paiva, Bruno, additional
Published: 2018
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85. Introduction to the diagnosis and classification of monocytic-lineage leukemias by flow cytometry

Author: Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), Fundación Científica Asociación Española Contra el Cáncer, Junta de Castilla y León, Fundación Memoria de D. Samuel Solorzano Barruso, International Myeloma Foundation, Red Temática de Investigación Cooperativa en Cáncer (España), Matarraz, Sergio, Almeida, Julia, Flores-Montero, Juan, Lécrevisse, Quentin, Guerri, Valentina, López, Antonio, Barrena, Susana, Velden, Vincent H. J. van der, Marvelde, Jeroen G. te, Dongen, J. J. M. van, Orfao, Alberto, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), Fundación Científica Asociación Española Contra el Cáncer, Junta de Castilla y León, Fundación Memoria de D. Samuel Solorzano Barruso, International Myeloma Foundation, Red Temática de Investigación Cooperativa en Cáncer (España), Matarraz, Sergio, Almeida, Julia, Flores-Montero, Juan, Lécrevisse, Quentin, Guerri, Valentina, López, Antonio, Barrena, Susana, Velden, Vincent H. J. van der, Marvelde, Jeroen G. te, Dongen, J. J. M. van, and Orfao, Alberto
Abstract: Despite diagnostic criteria are currently available for the distinct subtypes of monocytic-lineage neoplasias, a number of partially overlapping features still remain evident, which may hamper their differential diagnosis. An accurate identification and characterization of monocytic cells is of major relevance for the diagnosis and classification of these neoplasias. In this regard, as compared to other conventional techniques, flow cytometry has shown the highest sensitivity for detection of early monocytic commitment of (normal and neoplastic) bone marrow CD34 hematopoietic precursors as well as of monocytic aberrations and maturation blockades, which are frequently associated with clonal myeloid disorders. In the present paper we provide basic principles and criteria for multiparameter flow cytometry identification and characterization of bone marrow monocytic cells that contribute to an improved diagnostic and classification of monocytic lineage-associated acute leukemias in clinical settings, particularly when using the EuroFlow antibody panels.
Published: 2017

86. Utility of CD54, CD229, and CD319 for the Identification of Plasma Cells in Patients with Clonal Plasma Cell Diseases

Author: Pojero, Fanny, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Pérez, José J., Puig, Noemi, Paiva, Bruno, Böttcher, Sebastian, Dongen, J. J. M. van, Orfao, Alberto, Immunology, Instituto de Salud Carlos III, European Commission, Ministerio de Economía y Competitividad (España), International Myeloma Foundation, and Red Temática de Investigación Cooperativa en Cáncer (España)
Subjects: immune system diseases, hemic and lymphatic diseases
Abstract: [Background]: Multiparameter flow cytometry (MFC) identification and characterization of plasma cells (PCs) is a useful tool to support diagnosis, prognostication, and monitoring of PC diseases (PCD). Currently, the number of MFC markers suited for the identification of PC remains limited. Moreover, antibody therapies against PC-associated markers further compromise the utility of the most widely used reagents (e.g., CD38). Despite markers other than CD38 and CD138 are recognized as potentially useful PC-identification markers, no study has comparatively evaluated their performance in combination with CD38 and CD138. Here we compared the utility of CD229, CD54, and CD319 for the identification of normal and aberrant PCs. [Methods]: Bone marrow (BM) samples from 5 healthy controls, two noninfiltrated nonHodgkin lymphoma cases and 46 PCD patients plus 3 extraosseous plasmocytomas, and normal peripheral blood (PB) specimens, were studied. [Results]: Our results showed adequate performance of all three markers once combined with CD38. In contrast, when combined with CD138 for the identification of PC, only CD229 provided a good discrimination between PCs and all other cells for all BM and PB samples analyzed; in contrast, CD54 and CD319 showed limited utility for the identification of PCs, mainly because of significant overlap of the staining for these two markers on PCs and other myeloid cells in the sample. [Conclusions]: From the three markers evaluated, CD229 may be considered as the most reliable marker to replace CD38 or CD138 for the identification of PCs in patients undergoing anti-CD38 or anti-CD138 therapy, until a better alternative is available., Grant sponsor: the Instituto de Salud Carlos III (Ministry of Economy and Competitivity, Madrid, Spain); Grant number: FEDER (RD12/0036/0048; Grant sponsors: EuroFlow Consortium, the International Myeloma Foundation-Black Swan Research Initiative, the Red Tematica de Investigacion Cooperativa en Cancer (RTICC)
Published: 2016

87. Nuevas estrategias metodológicas y de análisis de datos de citrometría de flujo aplicadas al diagnóstico y clasificación de las hemopatías malignas

Author: Flores Montero, Juan Alejandro and Orfao de Matos Correia e Vale, José Alberto
Subjects: Enfermedades de la sangre, Academic dissertations, 3207.08 Hematología, Universidad de Salamanca (España), Citometría de flujo, 2407.04 Citología, Tesis y disertaciones académicas
Abstract: Tesis por compendio de publicaciones, [ES] Hoy en día el diágnostico y clasificación de las hemopatías malignas se asienta sobre las características citomorfológicas e histopatológicas del tumor, el inmunofenotipo de las células tumorales y sus características genéticas y moleculares, consideradas en el contexto del comportamiento clínico de la enfermedad.
Published: 2016

88. Impact of Next-Generation Flow (NGF) Minimal Residual Disease (MRD) Monitoring in Multiple Myeloma (MM): Results from the Pethema/GEM2012 Trial

Author: Paiva, Bruno, primary, Puig, Noemi, additional, Cedena, Maria Teresa, additional, Cordon, Lourdes, additional, Vidriales, Maria-Belen, additional, Burgos, Leire, additional, Flores-Montero, Juan, additional, Lopez-Anglada, Lucía, additional, Gutierrez, Norma, additional, Calasanz, Maria Jose, additional, Martin-Ramos, Maria Luisa, additional, Garcia-Sanz, Ramon, additional, Martinez-Lopez, Joaquin, additional, Oriol, Albert, additional, Blanchard, M Jesús, additional, Rios, Rafael, additional, Martín, Jesús, additional, Martínez, Rafael, additional, Sarra, Josep, additional, Hernández, Miguel T, additional, de la Rubia, Javier, additional, Krsnik, Isabel, additional, Moraleda, Jose M, additional, Palomera, Luis, additional, Bargay, Juan, additional, Orfao, Alberto, additional, Rosinol, Laura, additional, Mateos, Maria-Victoria, additional, Lahuerta, Juan-José, additional, Bladé, Joan, additional, and San Miguel, Jesus F., additional
Published: 2017
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89. Quality assessment program for EuroFlow protocols: Summary results of four-year (2010-2013) quality assurance rounds

Author: Kalina, Tomas, Flores-Montero, Juan, Lécrevisse, Quentin, Pedreira, C. E., Böttcher, Sebastian, Lima, Margarida, Langerak, Anton W., Martín-Ayuso, Marta, Dongen, J. J. M. van, Orfao, Alberto, Conselho Nacional de Desenvolvimento Científico e Tecnológico (Brasil), Fundação Carlos Chagas Filho de Amparo à Pesquisa do Estado do Rio de Janeiro, Red Temática de Investigación Cooperativa en Cáncer (España), Junta de Castilla y León, Ministry of Health of the Czech Republic, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, and Ministerio de Ciencia e Innovación (España)
Subjects: Leukemia, Lymphoma, EuroFlow, Flow cytometry, Quality assessment, Immunophenotyping
Abstract: Flow cytometric immunophenotyping has become essential for accurate diagnosis, classification, and disease monitoring in hemato-oncology. The EuroFlow Consortium has established a fully standardized >all-in-one> pipeline consisting of standardized instrument settings, reagent panels, and sample preparation protocols and software for data analysis and disease classification. For its reproducible implementation, parallel development of a quality assurance (QA) program was required. Here, we report on the results of four consecutive annual rounds of the novel external QA EuroFlow program. The novel QA scheme aimed at monitoring the whole flow cytometric analysis process (cytometer setting, sample preparation, acquisition and analysis) by reading the median fluorescence intensities (MedFI) of defined lymphocytes' subsets. Each QA participant applied the predefined reagents' panel on blood cells of local healthy donors. A uniform gating strategy was applied to define lymphocyte subsets and to read MedFI values per marker. The MedFI values were compared with reference data and deviations from reference values were quantified using performance score metrics. In four annual QA rounds, we analyzed 123 blood samples from local healthy donors on 14 different instruments in 11 laboratories from nine European countries. The immunophenotype of defined cellular subsets appeared sufficiently standardized to permit unified (software) data analysis. The coefficient of variation of MedFI for 7 of 11 markers performed repeatedly below 30%, average MedFI in each QA round ranged from 86 to 125% from overall median. Calculation of performance scores was instrumental to pinpoint standardization failures and their causes. Overall, the new EuroFlow QA system for the first time allowed to quantify the technical variation that is introduced in the measurement of fluorescence intensities in a multicentric setting over an extended period of time. EuroFlow QA is a proficiency test specific for laboratories that use standardized EuroFlow protocols. It may be used to complement, but not replace, established proficiency tests., Funded by: European Commission . Grant Number: LSB-CT-2006–018708 (to EuroFlow Consortium); International Society of Advancement of Cytometry (“ISAC Scholar”; to T.K.); Ministry of Health of the Czech Republic . Grant Numbers: NT/12425 and NT/14534 (to T.K. , O.H. , E.M.); GAUK 802214 (to M.N.); CNPq- Brazilian National Research Council, (Brasília, Brazil) . Grant Number: Produtividade em Pesquisa: 305081/2011-0 and Universal: 472499/2012 (to C.E.P.); FAPERJ-Fundação de Amparo à Pesquisa do Rio de Janeiro, (Rio de Janeiro, Brazil) . Grant Number: (Cientista do Nosso Estado: E26/102.946/2011-CNE) (to C.E.P.); ERA-NET PRIOMEDCHILD . Grant Numbers: 40–41800-98-027 (to Ł.S. , T.S. , V.H.J.vd.V. , J.J.Mv.D.); Red de Cáncer (ISCIII-RTICC RD06/0020/0035 and RD12/036/048-FEDER, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad, Madrid, Spain) and Spanish Network of Cancer Research Centers (ISCIII RTICC-RD06/0020/0035-FEDER and RD12/0036/0048-FEDER), FIS 08/90881 from the ‘Fondo de Investigación Sanitaria', Ministerio de Ciencia e Innovación (Madrid, Spain) . Grant Numbers: GR37 EDU/894/2009 , SA016- A-09; Consejería de Educación, Junta de Castilla y León (Valladolid, Spain) . Grant Numbers: PIB2010BZ-00565 , Dirección General de Cooperación Internacional y Relaciones Institucionales, Secretaría de Estado de Investigación, Ministerio de Ciencia e Innovación (Madrid, Spain) (to J.F.M., Q.L., A.O.)
Published: 2015

90. Circulating tumor cells for comprehensive and multiregional non-invasive genetic characterization of multiple myeloma

Author: Garcés, Juan-José, Bretones, Gabriel, Burgos, Leire, Valdes-Mas, Rafael, Puig, Noemi, Cedena, Maria-Teresa, Alignani, Diego, Rodriguez, Idoia, Puente, Diana Álvarez, Álvarez, Miguel-García, Goicoechea, Ibai, Rodriguez, Sara, Calasanz, Maria-Jose, Agirre, Xabier, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Rodriguez-Otero, Paula, Rios, Rafael, Martinez-Lopez, Joaquin, Millacoy, Pamela, Palomera, Luis, Del Orbe, Rafael, Pérez-Montaña, Albert, El Omri, Halima, Prosper, Felipe, Mateos, Maria-Victoria, Rosiñol, Laura, Blade, Joan, Lahuerta, Juan-Jose, Orfao, Alberto, Lopez-Otin, Carlos, San Miguel, Jesus F., and Paiva, Bruno
Abstract: Multiple myeloma (MM) patients undergo repetitive bone marrow (BM) aspirates for genetic characterization. Circulating tumor cells (CTCs) are detectable in peripheral blood (PB) of virtually all MM cases and are prognostic, but their applicability for noninvasive screening has been poorly investigated. Here, we used next-generation flow (NGF) cytometry to isolate matched CTCs and BM tumor cells from 53 patients and compared their genetic profile. In eight cases, tumor cells from extramedullary (EM) plasmacytomas were also sorted and whole-exome sequencing was performed in the three spatially distributed tumor samples. CTCs were detectable by NGF in the PB of all patients with MM. Based on the cancer cell fraction of clonal and subclonal mutations, we found that ~22% of CTCs egressed from a BM (or EM) site distant from the matched BM aspirate. Concordance between BM tumor cells and CTCs was high for chromosome arm-level copy number alterations (≥95%) though not for translocations (39%). All high-risk genetic abnormalities except one t(4;14) were detected in CTCs whenever present in BM tumor cells. Noteworthy, ≥82% mutations present in BM and EM clones were detectable in CTCs. Altogether, these results support CTCs for noninvasive risk-stratification of MM patients based on their numbers and genetic profile.
Published: 2020
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91. Minimal residual disease monitoring and immune profiling in multiple myeloma in elderly patients

Author: Instituto de Salud Carlos III, Red Temática de Investigación Cooperativa en Cáncer (España), Asociación Española Contra el Cáncer, International Myeloma Foundation, European Research Council, Paiva, Bruno, Cedena, Maria-Teresa, Puig, Noemi, Arana, Paula, Vidriales, Maria Belén, Cordón, Lourdes, Flores-Montero, Juan, Gutiérrez, Norma Carmen, Martín-Ramos, María-Luisa, Martínez-López, Joaquín, Ocio, Enrique M., Hernandez, Miguel T., Teruel, Ana-Isabel, Rosiñol, Laura, Echeveste, María-Asunción, Martínez, Rafael, Gironella, Mercedes, Oriol, Albert, Cabrera, Carmen, Martín, Jesús, Bargay, Joan, Encinas, Cristina, González, Yolanda, Dongen, J. J. M. van, Orfao, Alberto, Bladé, Joan, Mateos, Maria Victoria, Lahuerta, Juan José, San Miguel, Jesús F., Instituto de Salud Carlos III, Red Temática de Investigación Cooperativa en Cáncer (España), Asociación Española Contra el Cáncer, International Myeloma Foundation, European Research Council, Paiva, Bruno, Cedena, Maria-Teresa, Puig, Noemi, Arana, Paula, Vidriales, Maria Belén, Cordón, Lourdes, Flores-Montero, Juan, Gutiérrez, Norma Carmen, Martín-Ramos, María-Luisa, Martínez-López, Joaquín, Ocio, Enrique M., Hernandez, Miguel T., Teruel, Ana-Isabel, Rosiñol, Laura, Echeveste, María-Asunción, Martínez, Rafael, Gironella, Mercedes, Oriol, Albert, Cabrera, Carmen, Martín, Jesús, Bargay, Joan, Encinas, Cristina, González, Yolanda, Dongen, J. J. M. van, Orfao, Alberto, Bladé, Joan, Mateos, Maria Victoria, Lahuerta, Juan José, and San Miguel, Jesús F.
Abstract: The value of minimal residual disease (MRD) in multiple myeloma (MM) has been more frequently investigated in transplant-eligible patients than in elderly patients. Because an optimal balance between treatment efficacy and toxicity is of utmost importance in patients with elderly MM, sensitive MRD monitoring might be particularly valuable in this patient population. Here, we used second-generation 8-color multiparameter-flow cytometry (MFC) to monitor MRD in 162 transplant-ineligible MM patients enrolled in the PETHEMA/GEM2010MAS65 study. The transition from first- to second-generation MFC resulted in increased sensitivity and allowed us to identify 3 patient groups according to MRD levels: MRD negative (<10; n = 54, 34%), MRD positive (between <10 and ≥10; n = 20, 12%), and MRD positive (≥10; n = 88, 54%). MRD status was an independent prognostic factor for time to progression (TTP) (hazard ratio [HR], 2.7; P = .007) and overall survival (OS) (HR, 3.1; P = .04), with significant benefit for MRD-negative patients (median TTP not reached, 70% OS at 3 years), and similar poorer outcomes for cases with MRD levels between <10 and ≥10 vs ≥10 (both with a median TTP of 15 months; 63% and 55% OS at 3 years, respectively). Furthermore, MRD negativity significantly improved TTP of patients >75 years (HR, 4.8; P < .001), as well as those with high-risk cytogenetics (HR, 12.6; P = .01). Using second-generation MFC, immune profiling concomitant to MRD monitoring also contributed to identify patients with poor, intermediate, and favorable outcomes (25%, 61%, and 100% OS at 3 years, respectively; P = .01), the later patients being characterized by an increased compartment of mature B cells. Our results show that similarly to transplant candidates, MRD monitoring is one of the most relevant prognostic factors in elderly MM patients, irrespectively of age or cytogenetic risk.
Published: 2016

92. Utility of CD54, CD229, and CD319 for the identification of plasma cells in patients with clonal plasma cell diseases

Author: Instituto de Salud Carlos III, European Commission, Ministerio de Economía y Competitividad (España), International Myeloma Foundation, Red Temática de Investigación Cooperativa en Cáncer (España), Pojero, Fanny, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Pérez, José J., Puig, Noemi, Paiva, Bruno, Böttcher, Sebastian, Dongen, J. J. M. van, Orfao, Alberto, Instituto de Salud Carlos III, European Commission, Ministerio de Economía y Competitividad (España), International Myeloma Foundation, Red Temática de Investigación Cooperativa en Cáncer (España), Pojero, Fanny, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Pérez, José J., Puig, Noemi, Paiva, Bruno, Böttcher, Sebastian, Dongen, J. J. M. van, and Orfao, Alberto
Abstract: [Background]: Multiparameter flow cytometry (MFC) identification and characterization of plasma cells (PCs) is a useful tool to support diagnosis, prognostication, and monitoring of PC diseases (PCD). Currently, the number of MFC markers suited for the identification of PC remains limited. Moreover, antibody therapies against PC-associated markers further compromise the utility of the most widely used reagents (e.g., CD38). Despite markers other than CD38 and CD138 are recognized as potentially useful PC-identification markers, no study has comparatively evaluated their performance in combination with CD38 and CD138. Here we compared the utility of CD229, CD54, and CD319 for the identification of normal and aberrant PCs. [Methods]: Bone marrow (BM) samples from 5 healthy controls, two noninfiltrated nonHodgkin lymphoma cases and 46 PCD patients plus 3 extraosseous plasmocytomas, and normal peripheral blood (PB) specimens, were studied. [Results]: Our results showed adequate performance of all three markers once combined with CD38. In contrast, when combined with CD138 for the identification of PC, only CD229 provided a good discrimination between PCs and all other cells for all BM and PB samples analyzed; in contrast, CD54 and CD319 showed limited utility for the identification of PCs, mainly because of significant overlap of the staining for these two markers on PCs and other myeloid cells in the sample. [Conclusions]: From the three markers evaluated, CD229 may be considered as the most reliable marker to replace CD38 or CD138 for the identification of PCs in patients undergoing anti-CD38 or anti-CD138 therapy, until a better alternative is available.
Published: 2016

93. Circulating Tumor Cells (CTCs) for Comprehensive and Multiregional Non-Invasive Genetic Characterization of Multiple Myeloma (MM)

Author: Garcés, Juan José, Bretones, Gabriel, Burgos, Leire, Valdés-Mas, Rafael, Alignani, Diego, Puente, Diana Álvarez, Goicoechea, Ibai, García-Álvarez, Miguel, Garate, Sonia, Rodríguez, Idoia, Calasanz, Maria-Jose, Rodríguez-Otero, Paula, Tamayo, Rafael Ríos, Martinez-Lopez, Joaquin, Millacoy, Pamela, Bernal, Luis Palomera, Del Orbe, Rafael, Montaña, Albert Pérez, Agirre, Xabier, Flores-Montero, Juan, Sanoja-Flores, Luzalba, Orfao, Alberto, El Omri, Halima, Prosper, Felipe, López-Otín, Carlos, San-Miguel, Jesus, and Paiva, Bruno
Published: 2019
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94. Expression profile of novel cell surface molecules on different subsets of human peripheral blood antigen-presenting cells

Author: Damasceno, Daniela, primary, Andrés, Martín Pérez, additional, van den Bossche, Wouter BL, additional, Flores-Montero, Juan, additional, de Bruin, Sandra, additional, Teodosio, Cristina, additional, van Dongen, Jacques JM, additional, Orfao, Alberto, additional, and Almeida, Julia, additional
Published: 2016
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95. Quality assessment program for EuroFlow protocols: Summary results of four-year (2010-2013) quality assurance rounds

Author: Conselho Nacional de Desenvolvimento Científico e Tecnológico (Brasil), Fundação Carlos Chagas Filho de Amparo à Pesquisa do Estado do Rio de Janeiro, Red Temática de Investigación Cooperativa en Cáncer (España), Junta de Castilla y León, Ministry of Health of the Czech Republic, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Ministerio de Ciencia e Innovación (España), Kalina, Tomas, Flores-Montero, Juan, Lécrevisse, Quentin, Pedreira, C. E., Böttcher, Sebastian, Lima, Margarida, Langerak, Anton W., Martín-Ayuso, Marta, Dongen, J. J. M. van, Orfao, Alberto, Conselho Nacional de Desenvolvimento Científico e Tecnológico (Brasil), Fundação Carlos Chagas Filho de Amparo à Pesquisa do Estado do Rio de Janeiro, Red Temática de Investigación Cooperativa en Cáncer (España), Junta de Castilla y León, Ministry of Health of the Czech Republic, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Ministerio de Ciencia e Innovación (España), Kalina, Tomas, Flores-Montero, Juan, Lécrevisse, Quentin, Pedreira, C. E., Böttcher, Sebastian, Lima, Margarida, Langerak, Anton W., Martín-Ayuso, Marta, Dongen, J. J. M. van, and Orfao, Alberto
Abstract: Flow cytometric immunophenotyping has become essential for accurate diagnosis, classification, and disease monitoring in hemato-oncology. The EuroFlow Consortium has established a fully standardized >all-in-one> pipeline consisting of standardized instrument settings, reagent panels, and sample preparation protocols and software for data analysis and disease classification. For its reproducible implementation, parallel development of a quality assurance (QA) program was required. Here, we report on the results of four consecutive annual rounds of the novel external QA EuroFlow program. The novel QA scheme aimed at monitoring the whole flow cytometric analysis process (cytometer setting, sample preparation, acquisition and analysis) by reading the median fluorescence intensities (MedFI) of defined lymphocytes' subsets. Each QA participant applied the predefined reagents' panel on blood cells of local healthy donors. A uniform gating strategy was applied to define lymphocyte subsets and to read MedFI values per marker. The MedFI values were compared with reference data and deviations from reference values were quantified using performance score metrics. In four annual QA rounds, we analyzed 123 blood samples from local healthy donors on 14 different instruments in 11 laboratories from nine European countries. The immunophenotype of defined cellular subsets appeared sufficiently standardized to permit unified (software) data analysis. The coefficient of variation of MedFI for 7 of 11 markers performed repeatedly below 30%, average MedFI in each QA round ranged from 86 to 125% from overall median. Calculation of performance scores was instrumental to pinpoint standardization failures and their causes. Overall, the new EuroFlow QA system for the first time allowed to quantify the technical variation that is introduced in the measurement of fluorescence intensities in a multicentric setting over an extended period of time. EuroFlow QA is a proficiency test specific for la
Published: 2015

96. CD117 expression in gammopathies is associated with an altered maturation of the myeloid and lymphoid hematopoietic cell

Author: Schmidt-Hieber, M., Pérez-Andrés, Martin, Paiva, Bruno, Flores-Montero, Juan, Gutiérrez, Norma Carmen, Matarraz, Sergio, San Miguel, Jesús F., and Orfao, Alberto
Subjects: Lymphoid Maturation, Multiparameter Flow Cytometry, Myeloid Maturation, Monoclonal Gammopathy, CD117 Expression, Normal Residual Plasma Cells, digestive system diseases
Abstract: 5 páginas, 1 figura, 2 tablas.-- et al., Aberrant CD117 expression is associated with a favorable outcome in multiple myeloma. We analyzed 106 patients with symptomatic multiple myeloma (n=50), smoldering multiple myeloma (n=38) and monoclonal gammopathy of undetermined significance (n=18) to elucidate biological features of CD117+ versus CD117− monoclonal gammopathies. CD117+ (mono)clonal plasma cells were detected in 30% symptomatic multiple myeloma, 45% smoldering multiple myeloma and 72% monoclonal gammopathy of undetermined significance patients. CD117 expression was associated with higher percentages of normal bone marrow plasma cells, CD117+ myeloid precursors and CD38+ B lymphocytes in all monoclonal gammopathies. Conversely, the number of bone marrow CD34+ myeloid cells and peripheral blood neutrophils was reduced among CD117+ multiple myeloma but not monoclonal gammopathy of undetermined significance patients. CD117 expression by (mono)clonal plasma cells is associated with uniquely altered patterns of production of hematopoietic bone marrow cells with decreased peripheral blood neutrophil counts and persistence of normal residual bone marrow plasma cells., this work was supported by the Cooperative Research Thematic Network (RTICs; RTICC RD06/0020/0035, RD06/0020/0006 and G03/136), MM Jevitt, SL firm, Instituto de Salud Carlos III/Subdirección General de Investigación Sanitaria (FIS: PI060339; 02/0905; 01/0089/01-02; PS09/01897) and Gerencia Regional de Salud de Castilla y León; Ayuda de Excelencia de Castilla y León, Consejeria de Educación (EDU/894/2009, GR37), and Consejería de Sanidad (557/A/10), Junta de Castilla y León, Valladolid, Spain. This work was further supported by a grant from the Dr. Werner Jackstädt-Foundation (Wuppertal, Germany).
Published: 2011

97. Flow cytometric detection of BCR-ABL fusion proteins in leukemia patients via an immunobead assay

Author: Weerkamp, F., Flores-Montero, Juan, and Orfao, Alberto
Abstract: EuroFlow Open Workshop in Rio de Janeiro del 25 al 27 de Agosto de 2011.-- et al.
Published: 2011

98. Comparison Between First-Generation 4-Color Vs. Second-Generation 8-Color Multiparameter Flow Cytometry (MFC) to Monitor Minimal Residual Disease (MRD) in Multiple Myeloma (MM)

Author: Arana, Paula, primary, Paiva, Bruno, additional, Vidriales, Maria Belen, additional, Flores-Montero, Juan A, additional, Puig, Noemi, additional, Cedena, Teresa, additional, Cordon, Lourdes, additional, Martinez-López, Joaquin, additional, Ocio, Enrique M., additional, Hernandez, Miguel T, additional, Teruel, Ana Isabel, additional, Gironella, Mercedes, additional, Echeveste, M Asuncion, additional, Rosiñol, Laura, additional, Blade, Joan, additional, Lahuerta, Juan Jose, additional, van Dongen, Jacques J.M., additional, Orfao, Alberto, additional, Mateos, Maria-Victoria, additional, and San Miguel, Jesus, additional
Published: 2015
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99. Next Generation Flow (NGF): A High Sensitive Technique to Detect Circulating Peripheral Blood (PB) Clonal Plasma Cells (cPC) in Patients with Newly Diagnosed of Plasma Cell Neoplasms (PCN)

Author: Sanoja-Flores, *Luzalba, primary, Paiva, *Bruno, additional, Flores-Montero, Juan A, additional, Puig, Noemi, additional, Burgos, Leire, additional, García, Omar, additional, Prosper, Felipe, additional, Merino, Juana, additional, Vidriales, Maria Belen, additional, Mateos, Maria-Victoria, additional, Garcia, Ramon, additional, Palomera, Luis, additional, Rios, Rafael, additional, Cañizo, María Consuelo, additional, Durie, Brian G M, additional, van Dongen, Jacques J.M., additional, San Miguel, Jesus, additional, and Orfao, Alberto, additional
Published: 2015
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100. Next Generation Flow (NGF) for High Sensitive Detection of Minimal Residual Disease (MRD) in Multiple Myeloma (MM)

Author: Flores-Montero, Juan A, primary, Paiva, Bruno, additional, Sanoja-Flores, Luzalba, additional, Puig, Noemi, additional, García, Omar, additional, Böttcher, Sebastian, additional, Pérez-Morán, José J, additional, Vidriales, Maria Belen, additional, Mateos, Maria-Victoria, additional, Garcia-Sanz, Ramon, additional, Jimenez, Cristina, additional, González, Marcos, additional, Martinez-López, Joaquin, additional, Cañizo, María Consuelo, additional, San Miguel, Jesus, additional, Durie, Brian, additional, van Dongen, Jacques J.M., additional, and Orfao, Alberto, additional
Published: 2015
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