Your search keyword '"Morán-Plata, F. Javier"' showing total 5 results

1. A novel NKp80-based strategy for universal identification of normal, reactive and tumor/clonal natural killer-cells in blood.

Author

Morán-Plata, F. Javier, Muñoz-García, Noemí, González-González, María, Pozo, Julio, Carretero-Domínguez, Sonia, Mateos, Sheila, Barrena, Susana, Belhassen-García, Moncef, Lau, Catarina, Dos Anjos Teixeira, Maria, Santos, Ana Helena, Yeguas, Ana, Balanzategui, Ana, García-Sancho, Alejandro Martín, Orfao, Alberto, and Almeida, Julia

Subjects

LYMPHOPROLIFERATIVE disorders, T cells, FLOW cytometry, TUMORS, DOWNREGULATION

Abstract

Purpose: Natural killer (NK) cells are traditionally identified by flow cytometry using a combination of markers (CD16/CD56/CD3), because a specific NK-cell marker is still missing. Here we investigated the utility of CD314, CD335 and NKp80, compared to CD16/CD56/CD3, for more robust identification of NK-cells in human blood, for diagnostic purposes. Methods: A total of 156 peripheral blood (PB) samples collected from healthy donors (HD) and patients with diseases frequently associated with loss/ downregulation of classical NK-cell markers were immunophenotyped following EuroFlow protocols, aimed at comparing the staining profile of total blood NK-cells for CD314, CD335 and NKp80, and the performance of distinct marker combinations for their accurate identification. Results: NKp80 showed a superior performance (vs. CD314 and CD335) for the identification of NK-cells in HD blood. Besides, NKp80 improved the conventional CD16/CD56/CD3-based strategy to identify PB NK-cells in HD and reactive processes, particularly when combined with CD16 for further accurate NK-cell-subsetting. Although NKp80+CD16 improved the identification of clonal/tumor NK-cells, particularly among CD56- cases (53%), aberrant downregulation of NKp80 was observed in 25% of patients, in whom CD56 was useful as a complementary NK-cell marker. As NKp80 is also expressed on T-cells, we noted increased numbers of NKp80+ cytotoxic T-cells at the more advanced maturation stages, mostly in adults. Conclusion: Here we propose a new robust approach for the identification of PB NK-cells, based on the combination of NKp80 plus CD16. However, in chronic lymphoproliferative disorders of NK-cells, addition of CD56 is recommended to identify clonal NK-cells, due to their frequent aberrant NKp80- phenotype. [ABSTRACT FROM AUTHOR]

Published

2024

2. Immune cell kinetics and antibody response in COVID-19 patients with low-count monoclonal B-cell lymphocytosis

Author

Fundación Científica Asociación Española Contra el Cáncer, Associazione Italiana per la Ricerca sul Cancro, Instituto de Salud Carlos III, Ministerio de Ciencia e Innovación (España), European Commission, Junta de Castilla y León, Oliva-Ariza, Guillermo, Fuentes-Herrero, Blanca, Lécrevisse, Quentin, Carbonell, Cristina, Pérez-Pons, Alba, Torres-Valle, Alba, Pozo, Julio, Martín-Oterino, José Ángel, González-López, Óscar, López-Bernús, Amparo, Bernal-Ribes, Marta, Belhassen-García, Moncef, Pérez-Escurza, Oihane, Pérez-Andrés, Martin, Vázquez, Lourdes, Hernández-Pérez, Guillermo, García Palomo, Francisco Javier, Leoz, Pilar, Costa-Alba, Pilar, Pérez-Losada, Elena, Yeguas, Ana, Santos Sánchez, Miryam, García-Blázquez, Marta, Morán-Plata, F Javier, Damasceno, Daniela, Botafogo, Vitor, Muñoz-García, Noemí, Fluxa, Rafael, Dongen, J. J. M. van, Marcos, Miguel, Almeida, Julia, Orfao, Alberto, Fundación Científica Asociación Española Contra el Cáncer, Associazione Italiana per la Ricerca sul Cancro, Instituto de Salud Carlos III, Ministerio de Ciencia e Innovación (España), European Commission, Junta de Castilla y León, Oliva-Ariza, Guillermo, Fuentes-Herrero, Blanca, Lécrevisse, Quentin, Carbonell, Cristina, Pérez-Pons, Alba, Torres-Valle, Alba, Pozo, Julio, Martín-Oterino, José Ángel, González-López, Óscar, López-Bernús, Amparo, Bernal-Ribes, Marta, Belhassen-García, Moncef, Pérez-Escurza, Oihane, Pérez-Andrés, Martin, Vázquez, Lourdes, Hernández-Pérez, Guillermo, García Palomo, Francisco Javier, Leoz, Pilar, Costa-Alba, Pilar, Pérez-Losada, Elena, Yeguas, Ana, Santos Sánchez, Miryam, García-Blázquez, Marta, Morán-Plata, F Javier, Damasceno, Daniela, Botafogo, Vitor, Muñoz-García, Noemí, Fluxa, Rafael, Dongen, J. J. M. van, Marcos, Miguel, Almeida, Julia, and Orfao, Alberto

Abstract

Low-count monoclonal B-cell lymphocytosis (MBLlo) has been associated with an underlying immunodeficiency and has recently emerged as a new risk factor for severe COVID-19. Here, we investigated the kinetics of immune cell and antibody responses in blood during COVID-19 of MBLlo versus non-MBL patients. For this study, we analyzed the kinetics of immune cells in blood of 336 COVID-19 patients (74 MBLlo and 262 non-MBL), who had not been vaccinated against SARS-CoV-2, over a period of 43 weeks since the onset of infection, using high-sensitivity flow cytometry. Plasma levels of anti-SARS-CoV-2 antibodies were measured in parallel by ELISA. Overall, early after the onset of symptoms, MBLlo COVID-19 patients showed increased neutrophil, monocyte, and particularly, plasma cell (PC) counts, whereas eosinophil, dendritic cell, basophil, and lymphocyte counts were markedly decreased in blood of a variable percentage of samples, and with a tendency toward normal levels from week +5 of infection onward. Compared with non-MBL patients, MBLlo COVID-19 patients presented higher neutrophil counts, together with decreased pre-GC B-cell, dendritic cell, and innate-like T-cell counts. Higher PC levels, together with a delayed PC peak and greater plasma levels of anti-SARS-CoV-2-specific antibodies (at week +2 to week +4) were also observed in MBLlo patients. In summary, MBLlo COVID-19 patients share immune profiles previously described for patients with severe SARS-CoV-2 infection, associated with a delayed but more pronounced PC and antibody humoral response once compared with non-MBL patients.

Published

2023

3. Anti-TRBC1 Antibody-Based Flow Cytometric Detection of T-Cell Clonality: Standardization of Sample Preparation and Diagnostic Implementation

Author

Muñoz-García, Noemí, primary, Lima, Margarida, additional, Villamor, Neus, additional, Morán-Plata, F. Javier, additional, Barrena, Susana, additional, Mateos, Sheila, additional, Caldas, Carolina, additional, Balanzategui, Ana, additional, Alcoceba, Miguel, additional, Domínguez, Alejandro, additional, Gómez, Fabio, additional, Langerak, Anton W., additional, van Dongen, Jacques J. M., additional, Orfao, Alberto, additional, and Almeida, Julia, additional

Published

2021

4. High-Sensitive TRBC1-Based Flow Cytometric Assessment of T-Cell Clonality in Tαβ-Large Granular Lymphocytic Leukemia.

Author

Muñoz-García, Noemí, Morán-Plata, F. Javier, Villamor, Neus, Lima, Margarida, Barrena, Susana, Mateos, Sheila, Caldas, Carolina, van Dongen, Jacques J. M., Orfao, Alberto, and Almeida, Julia

Subjects

*FLOW cytometry, *GENE expression, *LYMPHOCYTIC leukemia, *IMMUNOPHENOTYPING, *T cells, *CELL lines, *LYMPHOCYTE count, *LONGITUDINAL method

Abstract

Simple Summary: TRBC1 expression analysis by flow cytometry (FCM) has been recently proved to be a useful, simple and fast approach to assessing Tαβ-cell clonality. The aim of this study was to validate the utility of this assay specifically for the diagnosis of T-cell clonality of T-large granular lymphocytic leukemias (T-LGLL), as more mature polyclonal Tαβ large granular lymphocytes (Tαβ-LGL) show broader TRBC1+/TRBC1− ratios vs. total Tαβ cells. Our results showed that a TRBC1-FCM assay is also a fast and easy method for detecting T-cell clonality in T-LGLL based on altered (increased or decreased) percentages of TRBC1+ Tαβ cells of LGL expansions (i.e., with lymphocytosis) suspected of T-LGLL, whereas in the absence of lymphocytosis (or in TαβCD4-LGLL), the detection of increased absolute cell-counts of more precisely defined subpopulations of T-LGL expressing individual TCRVβ families is required. Flow cytometric (FCM) analysis of the constant region 1 of the T-cell receptor β chain (TRBC1) expression for assessing Tαβ-cell clonality has been recently validated. However, its utility for the diagnosis of clonality of T-large granular lymphocytic leukemia (T-LGLL) needs to be confirmed, since more mature Tαβ cells (i.e., T-LGL normal-counterpart) show broader TRBC1+/TRBC1− ratios vs. total Tαβ cells. We compared the distribution and absolute counts of TRBC1+ and TRBC1− Tαβ-LGL in blood containing polyclonal (n = 25) vs. clonal (n = 29) LGL. Overall, polyclonal TRBC1+ or TRBC1− Tαβ-LGL ranged between 0.36 and 571 cells/μL (3.2–91% TRBC1+ cells), whereas the clonal LGL cases showed between 51 and 11,678 cells/μL (<0.9% or >96% TRBC1+ cells). Among the distinct TCRVβ families, the CD28− effector-memory and terminal-effector polyclonal Tαβ cells ranged between 0 and 25 TRBC1+ or TRBC1− cells/μL and between 0 and 100% TRBC1+ cells, while clonal LGL ranged between 32 and 5515 TRBC1+ or TRBC1− cells/μL, representing <1.6% or >98% TRBC1+ cells. Our data support the utility of the TRBC1-FCM assay for detecting T-cell clonality in expansions of Tαβ-LGL suspected of T-LGLL based on altered percentages of TRBC1+ Tαβ cells. However, in the absence of lymphocytosis or in the case of TαβCD4-LGL expansion, the detection of increased absolute cell counts by the TRBC1-FCM assay for more accurately defined subpopulations of Tαβ-LGL-expressing individual TCRVβ families, allows the detection of T-cell clonality, even in the absence of phenotypic aberrations. [ABSTRACT FROM AUTHOR]

Published

2022

5. Immune cell kinetics and antibody response in COVID-19 patients with low-count monoclonal B-cell lymphocytosis.

Author

Oliva-Ariza G, Fuentes-Herrero B, Lecrevisse Q, Carbonell C, Pérez-Pons A, Torres-Valle A, Pozo J, Martín-Oterino JÁ, González-López Ó, López-Bernús A, Bernal-Ribes M, Belhassen-García M, Pérez-Escurza O, Pérez-Andrés M, Vazquez L, Hernández-Pérez G, García Palomo FJ, Leoz P, Costa-Alba P, Pérez-Losada E, Yeguas A, Santos Sánchez M, García-Blázquez M, Morán-Plata FJ, Damasceno D, Botafogo V, Muñoz-García N, Fluxa R, van Dongen JJM, Marcos M, Almeida J, and Orfao A

Subjects

Humans, B-Lymphocytes, Antibody Formation, SARS-CoV-2, Antibodies, Viral, Lymphocytosis, Leukemia, Lymphocytic, Chronic, B-Cell diagnosis, COVID-19, Neoplasms, Plasma Cell, Precancerous Conditions

Abstract

Low-count monoclonal B-cell lymphocytosis (MBL lo ) has been associated with an underlying immunodeficiency and has recently emerged as a new risk factor for severe COVID-19. Here, we investigated the kinetics of immune cell and antibody responses in blood during COVID-19 of MBL lo versus non-MBL patients. For this study, we analyzed the kinetics of immune cells in blood of 336 COVID-19 patients (74 MBL lo and 262 non-MBL), who had not been vaccinated against SARS-CoV-2, over a period of 43 weeks since the onset of infection, using high-sensitivity flow cytometry. Plasma levels of anti-SARS-CoV-2 antibodies were measured in parallel by ELISA. Overall, early after the onset of symptoms, MBL lo COVID-19 patients showed increased neutrophil, monocyte, and particularly, plasma cell (PC) counts, whereas eosinophil, dendritic cell, basophil, and lymphocyte counts were markedly decreased in blood of a variable percentage of samples, and with a tendency toward normal levels from week +5 of infection onward. Compared with non-MBL patients, MBL lo COVID-19 patients presented higher neutrophil counts, together with decreased pre-GC B-cell, dendritic cell, and innate-like T-cell counts. Higher PC levels, together with a delayed PC peak and greater plasma levels of anti-SARS-CoV-2-specific antibodies (at week +2 to week +4) were also observed in MBL lo patients. In summary, MBL lo COVID-19 patients share immune profiles previously described for patients with severe SARS-CoV-2 infection, associated with a delayed but more pronounced PC and antibody humoral response once compared with non-MBL patients., (© 2023 The Authors. American Journal of Hematology published by Wiley Periodicals LLC.)

Published

2023