Your search keyword '"Jara-Acevedo M"' showing total 108 results

1. Complete response to gemtuzumab ozogamicin in a patient with refractory mast cell leukemia

Author

Alvarez-Twose, I, Martínez-Barranco, P, Gotlib, J, García-Montero, A, Morgado, J M, Jara-Acevedo, M, Merker, J D, Peñalver, F J, Matito, A, Hou, Y, Sánchez-Muñoz, L, Mayado, A, Mollejo, M, Escribano, L, and Orfao, A

Published

2016

2. Increased IL6 plasma levels in indolent systemic mastocytosis patients are associated with high risk of disease progression

Author

Mayado, A, Teodosio, C, Garcia-Montero, A C, Matito, A, Rodriguez-Caballero, A, Morgado, J M, Muñiz, C, Jara-Acevedo, M, Álvarez-Twose, I, Sanchez-Muñoz, L, Matarraz, S, Caldas, C, Muñoz-González, J I, Escribano, L, and Orfao, A

Published

2016

3. Immunophenotypic alterations of bone marrow myeloid cell compartments in multiple myeloma patients predict for myelodysplasia-associated cytogenetic alterations

Author

Matarraz, S, Paiva, B, Díez-Campelo, M, Bárrena, S, Jara-Acevedo, M, Gutiérrez, M L, Sayagués, J M, Sánchez, M-L, Bárcena, P, Garrastazul, M P, Berruezo, M J, Duran, J M, Cerveró, C, García-Erce, J A, Florensa, L, Méndez, G D, Gutierrez, O, del Cañizo, M C, van Dongen, J J M, San Miguel, J F, and Orfao, A

Published

2014

4. Newly diagnosed adult AML and MPAL patients frequently show clonal residual hematopoiesis

Author

Fernandez, C, Santos-Silva, M C, López, A, Matarraz, S, Jara-Acevedo, M, Ciudad, J, Gutierrez, M L, Sánchez, M L, Salvador-Osuna, C, Berruezo, M J, Díaz-Arias, J Á, Palomo-Hernández, A M, Colado, E, González, N, Gallardo, D, Asensio, A, García-Sánchez, R, Saldaña, R, Cerveró, C, Carboné-Bañeres, A, Gutierrez, O, and Orfao, A

Published

2013

5. An immature immunophenotype of bone marrow mast cells predicts for multilineage D816V KIT mutation in systemic mastocytosis

Author

Teodosio, C, García-Montero, A C, Jara-Acevedo, M, Álvarez-Twose, I, Sánchez-Muñoz, L, Almeida, J, Morgado, J M, Matito, A, Escribano, L, and Orfao, A

Published

2012

6. CLL-like B-lymphocytes are systematically present at very low numbers in peripheral blood of healthy adults

Author

Almeida, J, Nieto, W G, Teodosio, C, Pedreira, C E, López, A, Fernández-Navarro, P, Nieto, A, Rodríguez-Caballero, A, Muñoz-Criado, S, Jara-Acevedo, M, Romero, A, and Orfao, A

Published

2011

7. Validation of the REMA Score for Predicting Systemic Mastocytosis in Patients with Mast Cell Activation Disorders: 961

Author

Alvarez-Twose, I., González-de-Olano, D., Sánchez-Muñoz, L., Matito, A., Morgado, J., Jara-Acevedo, M., Teodosio, C., García-Montero, A., Orfao, A., and Escribano, L.

Published

2011

8. Characterization of CD34 + hematopoietic cells in systemic mastocytosis: Potential role in disease dissemination

Author

Mayado, A., primary, Teodosio, C., additional, Dasilva‐Freire, N., additional, Jara‐Acevedo, M., additional, Garcia‐Montero, A. C., additional, Álvarez‐Twose, I., additional, Sánchez‐Muñoz, L., additional, Matito, A., additional, Caldas, C., additional, Muñoz‐González, J. I., additional, Henriques, A., additional, Sánchez‐Gallego, J. I., additional, Escribano, L., additional, and Orfao, A., additional

Published

2018

9. Characterization of CD34+ hematopoietic cells in systemic mastocytosis: Potential role in disease dissemination.

Author

Mayado, A., Teodosio, C., Dasilva‐Freire, N., Jara‐Acevedo, M., Garcia‐Montero, A. C., Álvarez‐Twose, I., Sánchez‐Muñoz, L., Matito, A., Caldas, C., Muñoz‐González, J. I., Henriques, A., Sánchez‐Gallego, J. I., Escribano, L., and Orfao, A.

Subjects

HEMATOPOIETIC stem cells, MAST cell disease, LEUCOCYTES, BONE marrow, BLOOD, FLOW cytometry

Abstract

Abstract: Background: Recent studies show that most systemic mastocytosis (SM) patients, including indolent SM (ISM) with (ISMs+) and without skin lesions (ISMs−), carry the KIT D816V mutation in PB leukocytes. We investigated the potential association between the degree of involvement of BM hematopoiesis by the KIT D816V mutation and the distribution of different maturation‐associated compartments of bone marrow (BM) and peripheral blood (PB) CD34+ hematopoietic precursors (HPC) in ISM and identified the specific PB cell compartments that carry this mutation. Methods: The distribution of different maturation‐associated subsets of BM and PB CD34+ HPC from 64 newly diagnosed (KIT‐mutated) ISM patients and 14 healthy controls was analyzed by flow cytometry. In 18 patients, distinct FACS‐purified PB cell compartments were also investigated for the KIT mutation. Results: ISM patients showed higher percentages of both BM and PB MC‐committed CD34+ HPC vs controls, particularly among ISM cases with MC‐restricted KIT mutation (ISMMC); this was associated with progressive blockade of maturation of CD34+ HPC to the neutrophil lineage from ISMMC to multilineage KIT‐mutated cases (ISMML). Regarding the frequency of KIT‐mutated cases and cell populations in PB, variable patterns were observed, the percentage of KIT‐mutated PB CD34+ HPC, eosinophils, neutrophils, monocytes and T cells increasing from ISMs−MC and ISMs+MC to ISMML patients. Conclusion: The presence of the KIT D816V mutation in PB of ISM patients is associated with (early) involvement of circulating CD34+ HPC and multiple myeloid cell subpopulations, KIT‐mutated PB CD34+ HPC potentially contributing to early dissemination of the disease. [ABSTRACT FROM AUTHOR]

Published

2018

10. Mast cell-related disorders presenting with Kounis syndrome

Author

González-de-Olano, D., Matito, A., Sánchez-López, P., Sánchez-Muñoz, L., Morgado, J.M., Teodósio, C., Jara-Acevedo, M., García-Montero, A., Orfao, A., Escribano, L., Kounis, N.G., and Álvarez-Twose, I.

Published

2012

11. Increased IL6 plasma levels in indolent systemic mastocytosis patients are associated with high risk of disease progression

Author

Mayado, A, primary, Teodosio, C, additional, Garcia-Montero, A C, additional, Matito, A, additional, Rodriguez-Caballero, A, additional, Morgado, J M, additional, Muñiz, C, additional, Jara-Acevedo, M, additional, Álvarez-Twose, I, additional, Sanchez-Muñoz, L, additional, Matarraz, S, additional, Caldas, C, additional, Muñoz-González, J I, additional, Escribano, L, additional, and Orfao, A, additional

Published

2015

12. Circulating clonotypic B cells in multiple myeloma and monoclonal gammopathy of undetermined significance

Author

Thiago, L. S., primary, Perez-Andres, M., additional, Balanzategui, A., additional, Sarasquete, M. E., additional, Paiva, B., additional, Jara-Acevedo, M., additional, Barcena, P., additional, Sanchez, M. L., additional, Almeida, J., additional, Gonzalez, M., additional, San Miguel, J. F., additional, Garcia-Sanz, R., additional, and Orfao, A., additional

Published

2013

13. P-142 The proliferation index of bone marrow cells from myelodysplastic syndromes is associated with the diagnostic and prognostic of the disease

Author

Matarraz, S., primary, Teodosio, C., additional, Fernandez, C., additional, Albors, M., additional, Jara-Acevedo, M., additional, Lopez, A., additional, Gonzalez-Gonzalez, M., additional, Gutierrez, M.L., additional, Flores-Montero, J., additional, and Cervero, C., additional

Published

2013

14. An immature immunophenotype of bone marrow mast cells predicts for multilineage D816V KIT mutation in systemic mastocytosis

Author

Teodosio, C, primary, García-Montero, A C, additional, Jara-Acevedo, M, additional, Álvarez-Twose, I, additional, Sánchez-Muñoz, L, additional, Almeida, J, additional, Morgado, J M, additional, Matito, A, additional, Escribano, L, additional, and Orfao, A, additional

Published

2011

15. Validation of the REMA Score for Predicting Mast Cell Clonality and Systemic Mastocytosis in Patients with Systemic Mast Cell Activation Symptoms

Author

Alvarez-Twose, I., primary, González-de-Olano, D., additional, Sánchez-Muñoz, L., additional, Matito, A., additional, Jara-Acevedo, M., additional, Teodosio, C., additional, García-Montero, A., additional, Morgado, J.M., additional, Orfao, A., additional, and Escribano, L., additional

Published

2011

16. Indolent systemic mastocytosis without skin involvement vs. isolated bone marrow mastocytosis

Author

Escribano, L., primary, Alvarez-Twose, I., additional, Garcia-Montero, A., additional, Sanchez-Munoz, L., additional, Jara-Acevedo, M., additional, and Orfao, A., additional

Published

2011

17. Clinical, Biological And Molecular Characteristics Of Mast Cell Activation Disorders: A Prospective Study In 62 Patients By The Spanish Network On Mastocytosis (REMA).

Author

Alvarez-Twose, I., primary, González-Olano, D., additional, Sánchez-Muñoz, L., additional, Teodosio, C., additional, Jara-Acevedo, M., additional, Sánchez-Matas, I., additional, Matito, A., additional, García-Montero, A., additional, Orfao, A., additional, and Escribano, L., additional

Published

2009

18. Validation of the REMA Score for Predicting Mast Cell Clonality and Systemic Mastocytosis in Patients with Systemic Mast Cell Activation Symptoms.

Author

Alvarez-Twose, I., González-de-Olano, D., Sánchez-Muñoz, L., Matito, A., Jara-Acevedo, M., Teodosio, C., García-Montero, A., Morgado, J.M., Orfao, A., and Escribano, L.

Subjects

MAST cells, MAST cell disease, TRYPTASE, SYNCOPE, RECEIVER operating characteristic curves

Abstract

Background: A variable percentage of patients with systemic mast cell (MC) activation symptoms meet criteria for systemic mastocytosis (SM). We prospectively evaluated the clinical utility of the REMA score versus serum baseline tryptase (sBt) levels for predicting MC clonality and SM in 158 patients with systemic MC activation symptoms in the absence of mastocytosis in the skin (MIS). Methods: World Health Organization criteria for SM were applied in all cases. MC clonality was defined as the presence of KIT-mutated MC or by a clonal HUMARA test. The REMA score consisted of the assignment of positive or negative points as follows: male (+1), female (-1), sBt <15 μg/l (-1) or >25 μg/l (+2), presence (-2) or absence (+1) of pruritus, hives or angioedema and presence (+3) of presyncope or syncope. Efficiency of the REMA score for predicting MC clonality and SM was assessed by receiver operating characteristic (ROC) curve analyses and compared to those obtained by means of sBt levels alone. Results: Molecular studies revealed the presence of clonal MC in 68/80 SM cases and in 11/78 patients who did not meet the criteria for SM. ROC curve analyses confirmed the greater sensitivity and a similar specificity of the REMA score versus sBt levels (84 vs. 59% and 74 vs. 70% for MC clonality and 87 vs. 62% and 73 vs. 71% for SM, respectively). Conclusions: Our results confirm the clinical utility of the REMA score to predict MC clonality and SM in patients suffering from systemic MC activation symptoms without MIS. Copyright © 2011 S. Karger AG, Basel [ABSTRACT FROM AUTHOR]

Published

2012

19. Complete response after imatinib mesylate therapy in a patient with well-differentiated systemic mastocytosis.

Author

Alvarez-Twose I, González P, Morgado JM, Jara-Acevedo M, Sánchez-Muñoz L, Matito A, Mollejo M, Orfao A, and Escribano L

Published

2012

20. Altered B-cell, plasma cell, and antibody immune profiles in blood of patients with systemic mastocytosis.

Author

Pérez-Pons A, Henriques A, Contreras Sanfeliciano T, Jara-Acevedo M, Navarro-Navarro P, García-Montero AC, Álvarez-Twose I, Lecrevisse Q, Fluxa R, Sánchez-Muñoz L, Caldas C, Pozo J, González-López Ó, Pérez-Andrés M, Mayado A, and Orfao A

Abstract

Background: Systemic mastocytosis (SM) is a heterogeneous disease characterized by an expansion of KIT-mutated constitutively activated mast cells (MCs) that release MC mediators, which might act on the tumor microenvironment including other immune cells., Objective: To investigate the blood distribution of B-cell, plasma cell (PC), and antibody isotype compartments in patients with SM., Methods: We used spectral flow cytometry and the EuroFlow Immunomonitoring panel and Lymphocyte Screening Tube to quantify B cells, PCs, and their subsets in blood of 108 patients with SM (35 bone marrow mastocytosis [BMM] cases, 64 indolent SM [ISM] cases, 9 aggressive SM [ASM] cases) versus 117 age-matched healthy donors and paired bone marrow samples of 31 patients with SM versus 17 controls, respectively. In parallel, IgM, IgD, IgG, IgA, and IgE plasma levels were measured., Results: Compared with healthy donors, patients with SM showed increased immature B-cell production in bone marrow (P = .003) associated with greater release of pre-germinal center immature (P < .001) and naive CD5 + B lymphocytes (P < .001) to blood, but a pronounced decrease in PC counts of all different IgH isotypes and subclasses (P ≤ .001) together with overall increased IgM (P = .001) and IgD (P < .001) plasma levels. Different immune profiles were found per diagnostic subtype of disease with progressively greater counts in blood of immature B lymphocytes together with decreased IgMD + , IgG2 + , IgA1 + , and IgA2 + memory B cells (P ≤ .032) and elevated IgM (P = .017) plasma levels in cases of ASM, increased IgM (P = .001) and IgD (P = .001) plasma levels in ISM cases, and exacerbated IgE (P < .001) with decreased IgG (P = .008) plasma levels in BMM cases., Conclusions: Our results reveal a significant dysregulation of the B-cell and PC compartments in blood of patients with SM, consistent with distinctly altered antibody isotype profiles in plasma of patients with BMM versus ISM versus ASM., Competing Interests: Disclosure statement This study was supported by grants from Instituto de Salud Carlos III (ISCIII; Madrid, Spain) and co-funded by the European Union (grant numbers PI19/01166, PI22/01657, and CB16/12/00400 for the Biomedical Research Networking Center Consortium [CIBERONC] program) and the Subprograma Estatal de Infraestructuras de Investigación y Equipamiento Científico Técnico de 2019 del Ministerio de Ciencia, Innovación y Universidades (Madrid, Spain) co-funded by the European Union (grant number EQC2019-005419-P). A.P.-P. was supported by a grant from the Government of Castilla y León (Valladolid, Spain; Orden EDU/556/2019) co-funded by the European Regional Development Fund (FEDER BDNS, Identif.: 422058). P.N.-N. was supported by a grant from the Government of Castilla y León (Valladolid, Spain; Orden EDU/875/2021) co-funded by the European Social Fund (FEDER BDNS, Identif.: 540787). O.G.-L. was supported by a grant from ISCIII (PFIS: FI20/00116-AES 2017-2020, BOE 28/03/2019-Orden CNU/354/2019) co-funded by the European Union (European Social Fund Plus). A.M. was supported by the CIBERONC program (contract number PRF-2869). Disclosure of potential conflict of interest: The authors declare that they have no relevant conflicts of interest., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

21. T-cell immune profile in blood of systemic mastocytosis: Association with disease features.

Author

Pérez-Pons A, Teodosio C, Jara-Acevedo M, Henriques A, Navarro-Navarro P, García-Montero AC, Álvarez-Twose I, Lecrevisse Q, Fluxa R, Sánchez-Muñoz L, Caldas C, Pozo J, Martín S, Sanfeliciano TC, Pedreira CE, Botafogo V, González-López O, Mayado A, and Orfao A

Subjects

Humans, Male, Middle Aged, Female, Adult, Aged, T-Lymphocyte Subsets immunology, T-Lymphocyte Subsets metabolism, Immunophenotyping, Proto-Oncogene Proteins c-kit genetics, Young Adult, Mutation, Aged, 80 and over, Mast Cells immunology, Killer Cells, Natural immunology, Mastocytosis, Systemic immunology, Mastocytosis, Systemic diagnosis, Mastocytosis, Systemic blood

Abstract

Background: Systemic mastocytosis (SM) is a heterogeneous disease characterized by an expansion of KIT-mutated mast cells (MC). KIT-mutated MC display activated features and release MC mediators that might act on the tumour microenvironment and other immune cells. Here, we investigated the distribution of lymphocyte subsets in blood of patients with distinct subtypes of SM and determined its association with other disease features., Methods: We studied the distribution of TCD4 + and TCD4 - cytotoxic cells and their subsets, as well as total NK- and B cells, in blood of 115 SM patients-38 bone marrow mastocytosis (BMM), 67 indolent SM (ISM), 10 aggressive SM (ASM)- and 83 age-matched healthy donors (HD), using spectral flow cytometry and the EuroFlow Immunomonitoring panel, and correlated it with multilineage KIT D816V , the alpha-tryptasemia genotype (HαT) and the clinical manifestations of the disease., Results: SM patients showed decreased counts (vs. HD) of TCD4 - cytotoxic cells, NK cells and several functional subsets of TCD4 + cells (total Th1, Th2-effector memory, Th22-terminal effector and Th1-like Tregs), together with increased T-follicular-helper and Th1/Th17-like Treg counts, associated with different immune profiles per diagnostic subtype of SM, in multilineal versus MC-restricted KIT D816V and in cases with a HαT + versus HαT - genotype. Unique immune profiles were found among BMM and ISM patients with MC-restricted KIT D816V who displayed HαT, anaphylaxis, hymenoptera venom allergy, bone disease, pruritus, flushing and GI symptoms., Conclusion: Our results reveal altered T- and NK-cell immune profiles in blood of SM, which vary per disease subtype, the pattern of involvement of haematopoiesis by KIT D816V , the HαT genotype and specific clinical manifestations of the disease., (© 2024 The Authors. Allergy published by European Academy of Allergy and Clinical Immunology and John Wiley & Sons Ltd.)

Published

2024

22. Clinical impact of the TPSAB1 genotype in mast cell diseases: A REMA study in a cohort of 959 individuals.

Author

González-de-Olano D, Navarro-Navarro P, Muñoz-González JI, Sánchez-Muñoz L, Henriques A, de-Andrés-Martín A, Peralta-Arjonilla D, Mayado A, Jara-Acevedo M, García-Montero AC, Orfao A, and Álvarez-Twose I

Subjects

Humans, Mast Cells, Tryptases genetics, Genotype, Anaphylaxis epidemiology, Anaphylaxis genetics, Anaphylaxis diagnosis, Mastocytosis diagnosis, Mastocytosis epidemiology, Mastocytosis genetics, Mast Cell Activation Syndrome

Abstract

Background: A close association between hereditary alpha-tryptasemia (HAT) and mast cell (MC) disorders has been previously reported. However, the relationship between HAT and the diagnostic subtypes and clinical features of MC disorders still remains to be established., Objective: To determine the prevalence of HAT in healthy donors (HD) vs patients with different diagnostic subtypes of MC activation syndromes (MCAS) and mastocytosis, and its relationship with the clinical behavior of the disease., Methods: A total of 959 subjects were studied including 346 healthy donors (HD), 464 mastocytosis, and 149 non-clonal MCAS patients. Molecular studies to assess the TPSAB1 genotype were performed, and data on serum baseline tryptase (sBT) and basal MC-mediator release episodes and triggers of anaphylaxis were collected., Results: HAT was detected in 15/346 (4%) HD versus 43/149 (29%) non-clonal MCAS and 84/464 (18%) mastocytosis cases. Among mastocytosis, HAT was more frequently found in patients with MC-restricted KIT D816V (21% vs. 10% among multilineage KIT D816V patients; p = .008). Overall, median sBT was higher in cases presenting with HAT (28.9 vs. 24.5 ng/mL; p = .008), while no significant differences in sBT were observed among HAT + mastocytosis patients depending on the presence of 1 vs. ≥2 extra copies of the α-tryptase gene (44.1 vs. 35.2 ng/mL, p > .05). In turn, anaphylaxis was more frequently observed in HAT + versus HAT - mastocytosis patients (76% vs. 65%; p = .018), while HAT + and HAT - patients who did not refer anaphylaxis as the presenting symptom (n = 308) showed a similar prevalence of subsequent anaphylaxis (35% vs. 36%, respectively)., Conclusion: The frequency of HAT in MC disorders varies according to the diagnostic subtype of the disease. HAT does not imply a higher risk (and severity) of anaphylaxis in mastocytosis patients in whom anaphylaxis is not part of the presenting symptoms of the disease., (© 2023 European Academy of Allergy and Clinical Immunology and John Wiley & Sons Ltd.)

Published

2024

23. KITD816V mutation in blood for the diagnostic screening of systemic mastocytosis and mast cell activation syndromes.

Author

Navarro-Navarro P, Álvarez-Twose I, Pérez-Pons A, Henriques A, Mayado A, García-Montero AC, Sánchez-Muñoz L, González-López O, Matito A, Caldas C, Jara-Acevedo M, and Orfao A

Subjects

Adult, Humans, Proto-Oncogene Proteins c-kit genetics, Mast Cells, Mutation, Mastocytosis, Systemic diagnosis, Mastocytosis, Systemic genetics, Mast Cell Activation Syndrome, Mastocytosis diagnosis, Mastocytosis genetics

Abstract

Background: Current diagnostic algorithms for systemic mastocytosis (SM) rely on the detection of KITD816V in blood to trigger subsequent bone marrow (BM) investigations., Methods: Here, we correlated the KITD816V mutational status of paired blood and BM samples from 368 adults diagnosed with mast cell activation syndrome (MCAS) and mastocytosis and determined the potential utility of investigating KITD816V in genomic DNA from blood-purified myeloid cell populations to increase diagnostic sensitivity. In a subset of 69 patients, we further evaluated the kinetics of the KITD816V cell burden during follow-up and its association with disease outcome., Results: Our results showed a high correlation (P < .0001) between the KITD816V mutation burden in blood and BM (74% concordant samples), but with a lower mean of KITD816V-mutated cells in blood (P = .0004) and a high rate of discordant BM + /blood - samples particularly among clonal MCAS (73%) and BM mastocytosis (51%), but also in cutaneous mastocytosis (9%), indolent SM (15%), and well-differentiated variants of indolent SM (7%). Purification of different compartments of blood-derived myeloid cells was done in 28 patients who were BM mast cell (MC) + /blood - for KITD816V, revealing KITD816V-mutated eosinophils (56%), basophils (25%), neutrophils (29%), and/or monocytes (31%) in most (61%) patients. Prognostically, the presence of ≥3.5% KITD816V-mutated cells (P < .0001) and an unstable KITD816V mutation cell burden (P < .0001) in blood and/or BM were both associated with a significantly shortened progression-free survival (PFS)., Conclusions: These results confirm the high specificity but limited sensitivity of KITD816V analysis in whole blood for the diagnostic screening of SM and other primary MCAS, which might be overcome by assessing the mutation in blood-purified myeloid cell populations., (© 2022 The Authors. Allergy published by European Academy of Allergy and Clinical Immunology and John Wiley & Sons Ltd.)

Published

2023

24. Bone and Cytokine Markers Associated With Bone Disease in Systemic Mastocytosis.

Author

Rama TA, Henriques AF, Matito A, Jara-Acevedo M, Caldas C, Mayado A, Muñoz-González JI, Moreira A, Cavaleiro-Rufo J, García-Montero A, Órfão A, Sanchez-Muñoz L, and Álvarez-Twose I

Subjects

Biomarkers blood, Humans, Male, Female, Adolescent, Young Adult, Adult, Middle Aged, Aged, Cytokines blood, Mastocytosis, Systemic blood, Mastocytosis, Systemic complications, Mastocytosis, Systemic immunology, Bone Remodeling immunology, Bone Resorption etiology, Osteosclerosis complications

Abstract

Background: Mastocytosis encompasses a heterogeneous group of diseases characterized by tissue accumulation of clonal mast cells, which frequently includes bone involvement. Several cytokines have been shown to play a role in the pathogenesis of bone mass loss in systemic mastocytosis (SM), but their role in SM-associated osteosclerosis remains unknown., Objective: To investigate the potential association between cytokine and bone remodeling markers with bone disease in SM, aiming at identifying biomarker profiles associated with bone loss and/or osteosclerosis., Methods: A total of 120 adult patients with SM, divided into 3 age and sex-matched groups according to their bone status were studied: (1) healthy bone (n = 46), (2) significant bone loss (n = 47), and (3) diffuse bone sclerosis (n = 27). Plasma levels of cytokines and serum baseline tryptase and bone turnover marker levels were measured at diagnosis., Results: Bone loss was associated with significantly higher levels of serum baseline tryptase (P = .01), IFN-γ (P = .05), IL-1β (P = .05), and IL-6 (P = .05) versus those found in patients with healthy bone. In contrast, patients with diffuse bone sclerosis showed significantly higher levels of serum baseline tryptase (P < .001), C-terminal telopeptide (P < .001), amino-terminal propeptide of type I procollagen (P < .001), osteocalcin (P < .001), bone alkaline phosphatase (P < .001), osteopontin (P < .01), and the C-C Motif Chemokine Ligand 5/RANTES chemokine (P = .01), together with lower IFN-γ (P = .03) and RANK-ligand (P = .04) plasma levels versus healthy bone cases., Conclusions: SM with bone mass loss is associated with a proinflammatory cytokine profile in plasma, whereas diffuse bone sclerosis shows increased serum/plasma levels of biomarkers related to bone formation and turnover, in association with an immunosuppressive cytokine secretion profile., (Copyright © 2023 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2023

25. Mast Cell Activation Syndromes: Comparison Between Two Scoring Models to Predict for Mast Cell Clonality.

Author

Rama TA, Torrado I, Henriques AF, Sánchez-Muñoz L, Jara-Acevedo M, Navarro-Navarro P, Caldas C, Mayado A, Muñoz-González J, García-Montero A, Mollejo M, Redondo E, Garbán A, Moreira A, Órfão A, and Álvarez-Twose I

Subjects

Male, Humans, Middle Aged, Female, Mast Cells, Tryptases, Anaphylaxis diagnosis, Anaphylaxis genetics, Mast Cell Activation Syndrome, Mastocytosis diagnosis, Mastocytosis genetics, Mastocytosis, Systemic diagnosis, Mastocytosis, Systemic genetics, Mastocytosis, Systemic complications, Arthropod Venoms

Abstract

Background: The Red Española de Mastocitosis (Spanish Network on Mastocytosis) score (REMAs) and the National Institutes of Health idiopathic clonal anaphylaxis score (NICAS) were developed for more efficient screening of mast cell (MC) clonality in MC activation syndromes. In a limited idiopathic anaphylaxis case series, the NICAS showed higher accuracy compared with the REMAs., Objective: To compare the performance of the REMAs against the NICAS in the diagnosis of MC clonality., Methods: We compared the diagnostic value of the REMAs against the NICAS in 182 patients (63% men, median age 56 years) who presented with anaphylaxis triggered by Hymenoptera venom allergy (45%), drugs (15%), food (11%), idiopathic anaphylaxis (20%), and mixed causes (10%). KIT mutation was assessed in parallel in whole blood and bone marrow (BM) and, when negative, in highly purified BM MC. TPSAB1 was genotyped in a subset of 71 patients., Results: We found higher accuracy and rates of correctly classified patients for the REMAs (82% and 84%) compared with the NICAS (75% and 75%; P = .02 and P = .03, respectively), particularly among men (P = .05), patients with systemic mastocytosis (P = .05), those presenting anaphylaxis owing to any cause featuring urticaria (P = .04), cardiovascular symptoms (P = .02), and/or presyncope (P = .02) and those with a blood-negative/BM-positive KIT mutational profile (P = .002), but not hereditary α-tryptasemia-associated genotypes. Combined assessment of the REMAs and KIT D816V in blood yielded an overall improved classification efficiency of 86% versus 84% for REMAs., Conclusions: The combined use of the REMAs and blood detection of KIT D816V is recommended, but more sensitive blood-based molecular assays to detect KIT D816V are needed., (Copyright © 2022 American Academy of Allergy, Asthma & Immunology. Published by Elsevier Inc. All rights reserved.)

Published

2023

26. Altered innate immune profile in blood of systemic mastocytosis patients.

Author

Pérez-Pons A, Jara-Acevedo M, Henriques A, Navarro-Navarro P, García-Montero AC, Álvarez-Twose I, Pedreira CE, Sánchez-Muñoz L, Damasceno D, Caldas C, Muñoz-González JI, Matito A, Flores-Montero J, González-López O, Criado I, Mayado A, and Orfao A

Abstract

Background: Mast cells (MC) from systemic mastocytosis (SM) patients release MC mediators that lead to an altered microenvironment with potential consequences on innate immune cells, such as monocytes and dendritic cells (DC). Here we investigated the distribution and functional behaviour of different populations of blood monocytes and DC among distinct diagnostic subtypes of SM., Methods: Overall, we studied 115 SM patients - 45 bone marrow mastocytosis (BMM), 61 indolent SM (ISM), 9 aggressive SM (ASM)- and 32 healthy donors (HD). Spontaneous and in vitro -stimulated cytokine production by blood monocytes, and their plasma levels, together with the distribution of different subsets of blood monocytes and DCs, were investigated., Results: SM patients showed increased plasma levels and spontaneous production by blood monocytes of IL1β, IL6, IL8, TNFα and IL10, associated with an exhausted ability of LPS + IFNγ-stimulated blood monocytes to produce IL1β and TGFβ. SM (particularly ISM) patients also showed decreased counts of total monocytes, at the expense of intermediate monocytes and non-classical monocytes. Interestingly, while ISM and ASM patients had decreased numbers of plasmacytoid DC and myeloid DC (and their major subsets) in blood, an expansion of AXL + DC was specifically encountered in BMM cases., Conclusion: These results demonstrate an altered distribution of blood monocytes and DC subsets in SM associated with constitutive activation of functionally impaired blood monocytes and increased plasma levels of a wide variety of inflammatory cytokines, reflecting broad activation of the innate immune response in mastocytosis., Competing Interests: Authors declared no conflicts of interest., (© 2022 The Authors. Clinical and Translational Allergy published by John Wiley & Sons Ltd on behalf of European Academy of Allergy and Clinical Immunology.)

Published

2022

27. Frequency and prognostic impact of blood-circulating tumor mast cells in mastocytosis.

Author

Henriques A, Muñoz-González JI, Sánchez-Muñoz L, Matito A, Torres-Rivera L, Jara-Acevedo M, Caldas C, Mayado A, Pérez-Pons A, García-Montero AC, Álvarez-Twose I, and Orfao A

Subjects

Adult, Aged, Aged, 80 and over, Antigens, CD34 analysis, Female, Humans, Male, Mastocytosis blood, Middle Aged, Prognosis, Young Adult, Mast Cells pathology, Mastocytosis diagnosis, Neoplastic Cells, Circulating pathology

Abstract

Circulating tumor mast cells (CTMCs) have been identified in the blood of a small number of patients with advanced systemic mastocytosis (SM). However, data are limited about their frequency and prognostic impact in patients with MC activation syndrome (MCAS), cutaneous mastocytosis (CM) and nonadvanced SM. We investigated the presence of CTMCs and MC-committed CD34+ precursors in the blood of 214 patients with MCAS, CM, or SM using highly sensitive next-generation flow cytometry. CTMCs were detected at progressively lower counts in almost all patients with advanced SM (96%) and smoldering SM (SSM; 100%), nearly half of the patients (45%) with indolent SM (ISM), and a few patients (7%) with bone marrow (BM) mastocytosis but were systematically absent in patients with CM and MCAS (P < .0001). In contrast to CTMC counts, the number of MC-committed CD34+ precursors progressively decreased from MCAS, CM, and BM mastocytosis to ISM, SSM, and advanced SM (P < .0001). Clinically, the presence (and number) of CTMCs in blood of patients with SM in general and nonadvanced SM (ISM and BM mastocytosis) in particular was associated with more adverse features of the disease, poorer-risk prognostic subgroups as defined by the International Prognostic Scoring System for advanced SM (P < .0001) and the Global Prognostic Score for mastocytosis (P < .0001), and a significantly shortened progression-free survival (P < .0001) and overall survival (P = .01). On the basis of our results, CTMCs emerge as a novel candidate biomarker of disseminated disease in SM that is strongly associated with advanced SM and poorer prognosis in patients with ISM., (© 2022 by The American Society of Hematology.)

Published

2022

28. Whole-Exome Sequencing Reveals Recurrent but Heterogeneous Mutational Profiles in Sporadic WHO Grade 1 Meningiomas.

Author

González-Tablas M, Prieto C, Arandia D, Jara-Acevedo M, Otero Á, Pascual D, Ruíz L, Álvarez-Twose I, García-Montero AC, Orfao A, and Tabernero MD

Abstract

Human WHO grade 1 meningiomas are generally considered benign tumors; despite this, they account for ≈50% of all recurrent meningiomas. Currently, limited data exist about the mutational profiles of grade 1 meningiomas and patient outcome. We investigated the genetic variants present in 32 WHO grade 1 meningiomas using whole exome sequencing, and correlated gene mutational profiles with tumor cytogenetics and patient outcome. Overall, WHO grade 1 meningiomas harbored numerous and heterogeneous genetic variants, which most frequently affected the NF2 (47%) gene and to a less extent the PNMA6A (22%), TIGD1 (16%), SMO (13%), PTEN (13%), CREG2 (9%), EEF1A1 (6%), POLR2A (6%), ARID1B (3%), and FAIM3 (3%) genes. Notably, non-synonymous genetic variants of SMO and POLR2A were restricted to diploid meningiomas, whereas NF2 mutations were only found among tumors that showed -22/22q ─ (with or without a complex karyotype). Based on NF2 mutations and tumor cytogenetics, four genetic profiles were defined with an impact on patient recurrence-free survival (RFS). These included (1) two good-prognosis tumor subgroups-diploid meningiomas (n=9) and isolated -22/22q ─ associated with NF2 mutation (n=7)-with RFS rates at 10 y of 100%; and (2) two subgroups of poor-prognosis meningiomas-isolated -22/22q ─ without NF2 mutation (n=3) and tumors with complex karyotypes (n=11)-with a RFS rate at 10 y of 48% (p=0.003). Our results point out the existence of recurrent but heterogeneous mutational profiles in WHO grade 1 meningiomas which have an impact on patient outcome., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 González-Tablas, Prieto, Arandia, Jara-Acevedo, Otero, Pascual, Ruíz, Álvarez-Twose, García-Montero, Orfao and Tabernero.)

Published

2021

29. Proposed global prognostic score for systemic mastocytosis: a retrospective prognostic modelling study.

Author

Muñoz-González JI, Álvarez-Twose I, Jara-Acevedo M, Zanotti R, Perkins C, Jawhar M, Sperr WR, Shoumariyeh K, Schwaab J, Greiner G, Henriques A, Caldas C, Fernández-Giménez C, Sánchez-Muñoz L, Mayado A, Pérez-Pons A, Schmitt-Graeff A, Duyster J, Tanasi I, Olivieri F, Mora-Casterá E, Luna I, Senent L, Bañas MH, Nuñez-García A, Jurado-Chacón M, Martín-Sánchez G, Colado E, Xicoy B, Gener-Ricós G, Gotlib J, Bonadonna P, Reiter A, Valent P, García-Montero AC, and Orfao A

Subjects

Adult, Aged, Alkaline Phosphatase blood, Core Binding Factor Alpha 2 Subunit genetics, Female, Hemoglobins analysis, Humans, Kaplan-Meier Estimate, Male, Mastocytosis, Systemic mortality, Middle Aged, Polymorphism, Single Nucleotide, Prognosis, Progression-Free Survival, Repressor Proteins genetics, Retrospective Studies, Risk Factors, Serine-Arginine Splicing Factors genetics, Mastocytosis, Systemic diagnosis

Abstract

Background: Several risk stratification models have been proposed in recent years for systemic mastocytosis but have not been directly compared. Here we designed and validated a risk stratification model for progression-free survival (PFS) and overall survival (OS) in systemic mastocytosis on the basis of all currently available prognostic factors, and compared its predictive capacity for patient outcome with that of other risk scores., Methods: We did a retrospective prognostic modelling study based on patients diagnosed with systemic mastocytosis between March 1, 1983, and Oct 11, 2019. In a discovery cohort of 422 patients from centres of the Spanish Network on Mastocytosis (REMA), we evaluated previously identified, independent prognostic features for prognostic effect on PFS and OS by multivariable analysis, and designed a global prognostic score for mastocytosis (GPSM) aimed at predicting PFS (GPSM-PFS) and OS (GPSM-OS) by including only those variables that showed independent prognostic value (p<0·05). The GPSM scores were validated in an independent cohort of 853 patients from centres in Europe and the USA, and compared with pre-existing risk models in the total patient series (n=1275), with use of Harrells' concordance index (C-index) as a readout of the ability of each model to risk-stratify patients according to survival outcomes., Findings: Our GPSM-PFS and GPSM-OS models were based on unique combinations of independent prognostic factors for PFS (platelet count ≤100 × 10 9 cells per L, serum β2-microglobulin ≥2·5 μg/mL, and serum baseline tryptase ≥125 μg/L) and OS (haemoglobin ≤110 g/L, serum alkaline phosphatase ≥140 IU/L, and at least one mutation in SRSF2, ASXL1, RUNX1, or DNMT3A). The models showed clear discrimination between low-risk and high-risk patients in terms of worse PFS and OS prognoses in the discovery and validation cohorts, and further discrimination of intermediate-risk patients. The GPSM-PFS score was an accurate predictor of PFS in systemic mastocytosis (C-index 0·90 [95% CI 0·87-0·93], vs values ranging from 0·85 to 0·88 for pre-existing models), particularly in non-advanced systemic mastocytosis (C-index 0·85 [0·76-0·92], within the range for pre-existing models of 0·80 to 0·93). Additionally, the GPSM-OS score was able to accurately predict OS in the entire cohort (C-index 0·92 [0·89-0·94], vs 0·67 to 0·90 for pre-existing models), and showed some capacity to predict OS in advanced systemic mastocytosis (C-index 0·72 [0·66-0·78], vs 0·64 to 0·73 for pre-existing models)., Interpretation: All evaluated risk classifications predicted survival outcomes in systemic mastocytosis. The REMA-PFS and GPSM-PFS models for PFS, and the International Prognostic Scoring System for advanced systemic mastocytosis and GPSM-OS model for OS emerged as the most accurate models, indicating that robust prognostication might be prospectively achieved on the basis of biomarkers that are accessible in diagnostic laboratories worldwide., Funding: Carlos III Health Institute, European Regional Development Fund, Spanish Association of Mastocytosis and Related Diseases, Rare Diseases Strategy of the Spanish National Health System, Junta of Castile and León, Charles and Ann Johnson Foundation, Stanford Cancer Institute Innovation Fund, Austrian Science Fund., (Copyright © 2021 Elsevier Ltd. All rights reserved.)

Published

2021

30. STAT3 and STAT5B Mutations in T/NK-Cell Chronic Lymphoproliferative Disorders of Large Granular Lymphocytes (LGL): Association with Disease Features.

Author

Muñoz-García N, Jara-Acevedo M, Caldas C, Bárcena P, López A, Puig N, Alcoceba M, Fernández P, Villamor N, Flores-Montero JA, Gómez K, Lemes MA, Hernández JC, Álvarez-Twose I, Guerra JL, González M, Orfao A, and Almeida J

Abstract

STAT3 and STAT5B ( STAT3/STAT5B ) mutations are the most common mutations in T-cell large granular lymphocytic leukemia (T-LGLL) and chronic lymphoproliferative disorders of NK cells (CLPD-NK), but their clinical impact remains unknown. We investigated the frequency and type of STAT3/STAT5B mutations in FACS-sorted populations of expanded T/NK-LGL from 100 (82 clonal; 6 oligoclonal; 12 polyclonal) patients, and its relationship with disease features. Seventeen non-LGL T-CLPD patients and 628 age-matched healthy donors were analyzed as controls. STAT3 ( n = 30) and STAT5B ( n = 1) mutations were detected in 28/82 clonal T/NK-LGLL patients (34%), while absent (0/18, 0%) among oligoclonal/polyclonal LGL-lymphocytosis. Mutations were found across all diagnostic subgroups: TCD8 + -LGLL, 36%; CLPD-NK, 38%; TCD4 + -LGLL, 7%; Tαβ + DP-LGLL, 100%; Tαβ + DN-LGLL, 50%; Tγδ + -LGLL, 44%. STAT3 -mutated T-LGLL/CLPD-NK showed overall reduced ( p < 0.05) blood counts of most normal leukocyte subsets, with a higher rate (vs. nonmutated LGLL) of neutropenia ( p = 0.04), severe neutropenia ( p = 0.02), and cases requiring treatment ( p = 0.0001), together with a shorter time-to-therapy ( p = 0.0001), particularly in non-Y640F STAT3- mutated patients. These findings confirm and extend on previous observations about the high prevalence of STAT3 mutations across different subtypes of LGLL, and its association with a more marked decrease of all major blood-cell subsets and a shortened time-to-therapy.

Published

2020

31. Correction: Analysis of gene variants in the GASH/Sal model of epilepsy.

Author

Díaz-Casado E, Gómez-Nieto R, de Pereda JM, Muñoz LJ, Jara-Acevedo M, and López DE

Abstract

[This corrects the article DOI: 10.1371/journal.pone.0229953.].

Published

2020

32. Analysis of gene variants in the GASH/Sal model of epilepsy.

Author

Díaz-Casado E, Gómez-Nieto R, de Pereda JM, Muñoz LJ, Jara-Acevedo M, and López DE

Subjects

Acoustic Stimulation, Animals, Cricetinae, Disease Models, Animal, Epilepsy drug therapy, Epilepsy genetics, Epilepsy pathology, Epilepsy, Reflex drug therapy, Epilepsy, Reflex genetics, Epilepsy, Reflex pathology, Female, Gene Expression Regulation genetics, Guanine Nucleotide Exchange Factors genetics, Humans, Male, MutS Homolog 3 Protein genetics, Mutation genetics, Seizures drug therapy, Seizures genetics, Seizures pathology, Exome Sequencing, Computational Biology, Epilepsy epidemiology, Epilepsy, Reflex epidemiology, Seizures epidemiology

Abstract

Epilepsy is a complex neurological disorder characterized by sudden and recurrent seizures, which are caused by various factors, including genetic abnormalities. Several animal models of epilepsy mimic the different symptoms of this disorder. In particular, the genetic audiogenic seizure hamster from Salamanca (GASH/Sal) animals exhibit sound-induced seizures similar to the generalized tonic seizures observed in epileptic patients. However, the genetic alterations underlying the audiogenic seizure susceptibility of the GASH/Sal model remain unknown. In addition, gene variations in the GASH/Sal might have a close resemblance with those described in humans with epilepsy, which is a prerequisite for any new preclinical studies that target genetic abnormalities. Here, we performed whole exome sequencing (WES) in GASH/Sal animals and their corresponding controls to identify and characterize the mutational landscape of the GASH/Sal strain. After filtering the results, moderate- and high-impact variants were validated by Sanger sequencing, assessing the possible impact of the mutations by "in silico" reconstruction of the encoded proteins and analyzing their corresponding biological pathways. Lastly, we quantified gene expression levels by RT-qPCR. In the GASH/Sal model, WES showed the presence of 342 variations, in which 21 were classified as high-impact mutations. After a full bioinformatics analysis to highlight the high quality and reliable variants, the presence of 3 high-impact and 15 moderate-impact variants were identified. Gene expression analysis of the high-impact variants of Asb14 (ankyrin repeat and SOCS Box Containing 14), Msh3 (MutS Homolog 3) and Arhgef38 (Rho Guanine Nucleotide Exchange Factor 38) genes showed a higher expression in the GASH/Sal than in control hamsters. In silico analysis of the functional consequences indicated that those mutations in the three encoded proteins would have severe functional alterations. By functional analysis of the variants, we detected 44 significantly enriched pathways, including the glutamatergic synapse pathway. The data show three high-impact mutations with a major impact on the function of the proteins encoded by these genes, although no mutation in these three genes has been associated with some type of epilepsy until now. Furthermore, GASH/Sal animals also showed gene variants associated with different types of epilepsy that has been extensively documented, as well as mutations in other genes that encode proteins with functions related to neuronal excitability, which could be implied in the phenotype of the GASH/Sal. Our findings provide valuable genetic and biological pathway data associated to the genetic burden of the audiogenic seizure susceptibility and reinforce the need to validate the role of each key mutation in the phenotype of the GASH/Sal model., Competing Interests: The authors have declared that no competing interests exist.

Published

2020

33. Age Distribution of Multiple Functionally Relevant Subsets of CD4+ T Cells in Human Blood Using a Standardized and Validated 14-Color EuroFlow Immune Monitoring Tube.

Author

Botafogo V, Pérez-Andres M, Jara-Acevedo M, Bárcena P, Grigore G, Hernández-Delgado A, Damasceno D, Comans S, Blanco E, Romero A, Arriba-Méndez S, Gastaca-Abasolo I, Pedreira CE, van Gaans-van den Brink JAM, Corbiere V, Mascart F, van Els CACM, Barkoff AM, Mayado A, van Dongen JJM, Almeida J, and Orfao A

Subjects

Adolescent, Adult, Age Distribution, Aged, Aged, 80 and over, Blood Donors, Child, Child, Preschool, Female, Humans, Infant, Male, Middle Aged, Phenotype, Reproducibility of Results, T-Lymphocytes, Helper-Inducer immunology, T-Lymphocytes, Regulatory immunology, Young Adult, CD4-Positive T-Lymphocytes immunology, Fetal Blood cytology, Immunophenotyping methods, Monitoring, Immunologic methods

Abstract

CD4+ T cells comprise multiple functionally distinct cell populations that play a key role in immunity. Despite blood monitoring of CD4+ T-cell subsets is of potential clinical utility, no standardized and validated approaches have been proposed so far. The aim of this study was to design and validate a single 14-color antibody combination for sensitive and reproducible flow cytometry monitoring of CD4+ T-cell populations in human blood to establish normal age-related reference values and evaluate the presence of potentially altered profiles in three distinct disease models-monoclonal B-cell lymphocytosis (MBL), systemic mastocytosis (SM), and common variable immunodeficiency (CVID). Overall, 145 blood samples from healthy donors were used to design and validate a 14-color antibody combination based on extensive reagent testing in multiple cycles of design-testing-evaluation-redesign, combined with in vitro functional studies, gene expression profiling, and multicentric evaluation of manual vs. automated gating. Fifteen cord blood and 98 blood samples from healthy donors (aged 0-89 years) were used to establish reference values, and another 25 blood samples were evaluated for detecting potentially altered CD4 T-cell subset profiles in MBL ( n = 8), SM ( n = 7), and CVID ( n = 10). The 14-color tube can identify ≥89 different CD4+ T-cell populations in blood, as validated with high multicenter reproducibility, particularly when software-guided automated (vs. manual expert-based) gating was used. Furthermore, age-related reference values were established, which reflect different kinetics for distinct subsets: progressive increase of naïve T cells, T-helper (Th)1, Th17, follicular helper T (TFH) cells, and regulatory T cells (Tregs) from birth until 2 years, followed by a decrease of naïve T cells, Th2, and Tregs in older children and a subsequent increase in multiple Th-cell subsets toward late adulthood. Altered and unique CD4+ T-cell subset profiles were detected in two of the three disease models evaluated (SM and CVID). In summary, the EuroFlow immune monitoring TCD4 tube allows fast, automated, and reproducible identification of ≥89 subsets of CD4+ blood T cells, with different kinetics throughout life. These results set the basis for in-depth T-cell monitoring in different disease and therapeutic conditions., (Copyright © 2020 Botafogo, Pérez-Andres, Jara-Acevedo, Bárcena, Grigore, Hernández-Delgado, Damasceno, Comans, Blanco, Romero, Arriba-Méndez, Gastaca-Abasolo, Pedreira, van Gaans-van den Brink, Corbiere, Mascart, van Els, Barkoff, Mayado, van Dongen, Almeida and Orfao.)

Published

2020

34. Heterogeneous EGFR , CDK4 , MDM4 , and PDGFRA Gene Expression Profiles in Primary GBM: No Association with Patient Survival.

Author

González-Tablas M, Arandia D, Jara-Acevedo M, Otero Á, Vital AL, Prieto C, González-Garcia N, Nieto-Librero AB, Tao H, Pascual D, Ruiz L, Sousa P, Galindo-Villardón P, Orfao A, and Tabernero MD

Abstract

Background: The prognostic impact of the expression profile of genes recurrently amplified in glioblastoma multiforme (GBM) remains controversial., Methods: We investigated the RNA gene expression profile of epidermal growth factor receptor ( EGFR ), cyclin-dependent kinase 4 ( CDK4 ), murine doble minute 4 ( MDM4 ), and platelet derived growth factor receptor alpha ( PDGFRA ) in 83 primary GBM tumors vs. 42 normal brain tissue samples. Interphase FISH (iFISH) analysis for the four genes, together with analysis of intragenic deletions in EGFR and PDGFRA, were evaluated in parallel at the DNA level. As validation cohort, publicly available RNA gene expression data on 293 samples from 10 different GBM patient series were also studied., Results: At the RNA level, CDK4 was the most frequently overexpressed gene (90%) followed by EGFR (58%) and PDGFRA (58%). Chromosome 7 copy number alterations, i.e., trisomy (49%) and polysomy (44%), showed no clear association with EGFR gene expression levels. In turn, intragenic EGFR deletions were found in 39 patients (47%), including EGFRvIII (46%) in association with EGFRvIVa (4%), EGFRvII (2%) or other EGFR deletions (3%) and PDGFRA deletion of exons 8-9 was found in only two tumors (2%)., Conclusions: Overall, none of the gene expression profiles and/or intragenic EGFR deletions showed a significant impact on overall survival of GBM supporting the notion that other still unraveled features of the disease might play a more relevant prognostic role in GBM.

Published

2020

35. Complete Multilineage CD4 Expression Defect Associated With Warts Due to an Inherited Homozygous CD4 Gene Mutation.

Author

Fernandes RA, Perez-Andres M, Blanco E, Jara-Acevedo M, Criado I, Almeida J, Botafogo V, Coutinho I, Paiva A, van Dongen JJM, Orfao A, and Faria E

Subjects

CD4 Antigens blood, CD4-Positive T-Lymphocytes classification, CD4-Positive T-Lymphocytes immunology, CD4-Positive T-Lymphocytes pathology, Cell Lineage genetics, Cell Lineage immunology, Consanguinity, Cytotoxicity, Immunologic, Dendritic Cells immunology, Female, Genes, Recessive, Homozygote, Humans, Immunity, Humoral, Immunity, Innate, Immunophenotyping, Male, Middle Aged, Monocytes immunology, Pedigree, T-Lymphocytopenia, Idiopathic CD4-Positive pathology, Warts pathology, CD4 Antigens deficiency, CD4 Antigens genetics, Mutation, T-Lymphocytopenia, Idiopathic CD4-Positive genetics, T-Lymphocytopenia, Idiopathic CD4-Positive immunology, Warts genetics, Warts immunology

Abstract

Idiopathic T-CD4 lymphocytopenia (ICL) is a rare and heterogeneous syndrome characterized by opportunistic infections due to reduced CD4 T-lymphocytes (<300 cells/μl or <20% T-cells) in the absence of HIV infection and other primary causes of lymphopenia. Molecular testing of ICL has revealed defects in genes not specific to CD4 T-cells, with pleiotropic effects on other cell types. Here we report for the first time an absolute CD4 lymphocytopenia (<0.01 CD4 + T-cells/μl) due to an autosomal recessive CD4 gene mutation that completely abrogates CD4 protein expression on the surface membrane of T-cells, monocytes, and dendritic cells. A 45-year-old female born to consanguineous parents consulted because of exuberant, relapsing, and treatment-refractory warts on her hands and feet since the age of 10 years, in the absence of other recurrent infections or symptoms. Serological studies were negative for severe infections, including HIV 1/2, HTLV-1, and syphilis, but positive for CMV and EBV. Blood analysis showed the absence of CD4 + T-cells (<0.01%) with repeatedly increased counts of B-cells, naïve CD8 + T-lymphocytes, and particularly, CD4/CD8 double-negative (DN) TCRαβ + TCRγδ - T-cells (30% of T-cells; 400 cells/μl). Flow cytometric staining of CD4 using monoclonal antibodies directed against five different epitopes, located in two different domains of the protein, confirmed no cell surface membrane or intracytoplasmic expression of CD4 on T-cells, monocytes, and dendritic cells but normal soluble CD4 plasma levels. DN T-cells showed a phenotypic and functional profile similar to normal CD4 + T-cells as regards expression of maturation markers, T-helper and T-regulatory chemokine receptors, TCRvβ repertoire, and in vitro cytokine production against polyclonal and antigen-specific stimuli. Sequencing of the CD4 gene revealed a homozygous (splicing) mutation affecting the last bp on intron 7-8, leading to deletion of the juxtamembrane and intracellular domains of the protein and complete abrogation of CD4 expression on the cell membrane. These findings support previous studies in CD4 KO mice suggesting that surrogate DN helper and regulatory T-cells capable of supporting antigen-specific immune responses are produced in the absence of CD4 signaling and point out the need for better understanding the role of CD4 on thymic selection and the immune response., (Copyright © 2019 Fernandes, Perez-Andres, Blanco, Jara-Acevedo, Criado, Almeida, Botafogo, Coutinho, Paiva, van Dongen, Orfao and Faria.)

Published

2019

36. Frequency and prognostic impact of KIT and other genetic variants in indolent systemic mastocytosis.

Author

Muñoz-González JI, Álvarez-Twose I, Jara-Acevedo M, Henriques A, Viñas E, Prieto C, Sánchez-Muñoz L, Caldas C, Mayado A, Matito A, Dasilva-Freire N, Orfao A, and García-Montero AC

Subjects

Adolescent, Adult, Aged, Alleles, Biomarkers, Biomarkers, Tumor, Child, Child, Preschool, DNA Mutational Analysis, Female, Follow-Up Studies, Gene Frequency, Humans, Infant, Infant, Newborn, Male, Mastocytosis, Systemic diagnosis, Middle Aged, Mutation, Prognosis, Symptom Assessment, Young Adult, Genetic Variation, Mastocytosis, Systemic genetics, Mastocytosis, Systemic mortality, Proto-Oncogene Proteins c-kit genetics

Abstract

Indolent systemic mastocytosis (ISM) patients have a normal life expectancy, except in the 5% to 10% of cases that progress to more advanced SM (advSM), which has a significantly poorer outcome. Mutations in genes other than KIT frequently found in myeloid neoplasms have been associated with a poorer outcome among advSM, whereas limited information exists about their frequency and prognostic impact in ISM. We investigated the frequency and prognostic impact of variants in 18 genes, found to be altered in advSM, in 322 ISM patients (median follow-up, 5.7 years) divided into discovery (n = 200) and validation (n = 122) cohorts. Overall, 71 genetic variants were detected in 55 of 322 (17%) patients. Mutated ISM cases, particularly those carrying ASXL1 , RUNX1 , and/or DNMT3A ( A / R / D ) pathogenic variant allele frequencies (VAFs) ≥ 30%, exhibited significantly shortened ( P < .001) progression-free survival (PFS) and overall survival (OS). Multivariate analysis showed that serum β2-microglobulin (sβ2M) levels > 2.5 µg/mL (hazard ratio [HR], 9.8; P = .001), together with a KIT D816V VAF ≥ 1% in bone marrow (BM) (HR, 10.1; P = .02) and pathogenic variants of A / R / D VAFs ≥ 30% (HR, 4.2; P = .02), were the best combination of independent predictors for PFS. In turn, A / R / D gene pathogenic VAF ≥ 30% was the only independent predictor for OS (HR, 51.8; P < .001). Based on these variables, 2 scoring systems were constructed for risk stratification of ISM at diagnosis with significantly different 10-year PFS (100%, 91%, 0% for scores of 0, 1, ≥2, respectively) and OS (100% and 50% for scores of 0 and 1) rates., (© 2019 by The American Society of Hematology.)

Published

2019

37. Bone Marrow Mast Cell Antibody-Targetable Cell Surface Protein Expression Profiles in Systemic Mastocytosis.

Author

Dasilva-Freire N, Mayado A, Teodosio C, Jara-Acevedo M, Álvarez-Twose I, Matito A, Sánchez-Muñoz L, Caldas C, Henriques A, Muñoz-González JI, García-Montero AC, Sánchez-Gallego JI, Escribano L, and Orfao A

Subjects

Humans, Immunophenotyping, Mastocytosis, Systemic diagnosis, Prognosis, Antibodies metabolism, Bone Marrow Cells metabolism, Cell Membrane metabolism, Mast Cells metabolism, Mastocytosis, Systemic metabolism

Abstract

Despite recent therapeutic advances, systemic mastocytosis (SM) remains an incurable disease due to limited complete remission (CR) rates even after novel therapies. To date, no study has evaluated the expression on SM bone marrow mast cells (BMMC) of large panel of cell surface suitable for antibody-targeted therapy. In this study, we analyzed the expression profile of six cell-surface proteins for which antibody-based therapies are available, on BMMC from 166 SM patients vs. 40 controls. Overall, variable patterns of expression for the markers evaluated were observed among SM BMMC. Thus, CD22, CD30, and CD123, while expressed on BMMC from patients within every subtype of SM, showed highly variable patterns with a significant fraction of negative cases among advanced SM (aggressive SM (ASM), ASM with an associated clonal non-MC lineage disease (ASM-AHN) and MC leukemia (MCL)), 36%, 46%, and 39%, respectively. In turn, CD25 and FcεRI were found to be expressed in most cases (89% and 92%) in virtually all BMMC (median: 92% and 95%) from both indolent and advanced SM, but with lower/absent levels in a significant fraction of MC leukemia (MCL) and both in MCL and well-differentiated SM (WDSM) patients, respectively. In contrast, CD33 was the only marker expressed on all BMMC from every SM patient. Thus, CD33 emerges as the best potentially targetable cell-surface membrane marker in SM, particularly in advanced SM.

Published

2019

38. Impact of somatic and germline mutations on the outcome of systemic mastocytosis.

Author

Muñoz-González JI, Jara-Acevedo M, Alvarez-Twose I, Merker JD, Teodosio C, Hou Y, Henriques A, Roskin KM, Sanchez-Muñoz L, Tsai AG, Caldas C, Matito A, Sánchez-Gallego JI, Mayado A, Dasilva-Freire N, Gotlib JR, Escribano L, Orfao A, and García-Montero AC

Subjects

Adolescent, Adult, Aged, Alkaline Phosphatase blood, Bone Marrow Cells cytology, Bone Marrow Cells metabolism, Child, Disease-Free Survival, Female, Genetic Variation, Germ-Line Mutation, Hemoglobins analysis, Humans, Infant, Newborn, Male, Mastocytosis, Systemic genetics, Mastocytosis, Systemic mortality, Mastocytosis, Systemic pathology, Middle Aged, Neoplasm Staging, Polymorphism, Single Nucleotide, beta 2-Microglobulin blood, Mastocytosis, Systemic diagnosis, Proto-Oncogene Proteins c-kit genetics

Abstract

Systemic mastocytosis (SM) is a highly heterogeneous disease with indolent and aggressive forms, with the mechanisms leading to malignant transformation still remaining to be elucidated. Here, we investigated the presence and frequency of genetic variants in 34 SM patients with multilineal KIT D816V mutations. Initial screening was performed by targeted sequencing of 410 genes in DNA extracted from purified bone marrow cells and hair from 12 patients with nonadvanced SM and 8 patients with advanced SM, followed by whole-genome sequencing (WGS) in 4 cases. Somatic mutations were further investigated in another 14 patients with advanced SM. Despite the fact that no common mutation other than KIT D816V was found in WGS analyses, targeted next-generation sequencing identified 67 nonsynonymous genetic variants involving 39 genes. Half of the mutations were somatic (mostly multilineal), whereas the other half were germline variants. The presence of ≥1 multilineal somatic mutation involving genes other than KIT D816V, ≥3 germline variants, and ≥1 multilineal mutation in the SRSF2 , ASXL1 , RUNX1 , and/or EZH2 genes ( S/A/R/E genes), in addition to skin lesions, splenomegaly, thrombocytopenia, low hemoglobin levels, and increased alkaline phosphatase and β2-microglobulin serum levels, were associated with a poorer patient outcome. However, the presence of ≥1 multilineal mutation, particularly involving S/A/R/E genes, was the only independent predictor for progression-free survival and overall survival in our cohort., (© 2018 by The American Society of Hematology.)

Published

2018

39. KIT D816V Positive Acute Mast Cell Leukemia Associated with Normal Karyotype Acute Myeloid Leukemia.

Author

Lopes M, Teixeira MDA, Casais C, Mesquita V, Seabra P, Cabral R, Palla-García J, Lau C, Rodrigues J, Jara-Acevedo M, Freitas I, Vizcaíno JR, Coutinho J, Escribano L, Orfao A, and Lima M

Abstract

Introduction: Mast cell (MC) leukemia (MCL) is extremely rare. We present a case of MCL diagnosed concomitantly with acute myeloblastic leukemia (AML)., Case Report: A 41-year-old woman presented with asthenia, anorexia, fever, epigastralgia, and diarrhea. She had a maculopapular skin rash, hepatosplenomegaly, retroperitoneal adenopathies, pancytopenia, 6% blast cells (BC) and 20% MC in the peripheral blood, elevated lactate dehydrogenase, cholestasis, hypoalbuminemia, hypogammaglobulinemia, and increased serum tryptase (184  μ g/L). The bone marrow (BM) smears showed 24% myeloblasts, 17% promyelocytes, and 16% abnormal toluidine blue positive MC, and flow cytometry revealed 12% myeloid BC, 34% aberrant promyelocytes, a maturation blockage at the myeloblast/promyelocyte level, and 16% abnormal CD2-CD25+ MC. The BM karyotype was normal, and the KIT D816V mutation was positive in BM cells. The diagnosis of MCL associated with AML was assumed. The patient received corticosteroids, disodium cromoglycate, cladribine, idarubicin and cytosine arabinoside, high-dose cytosine arabinoside, and hematopoietic stem cell transplantation (HSCT). The outcome was favorable, with complete hematological remission two years after diagnosis and one year after HSCT., Conclusions: This case emphasizes the need of an exhaustive laboratory evaluation for the concomitant diagnosis of MCL and AML, and the therapeutic options.

Published

2018

40. Systemic mastocytosis with KIT V560G mutation presenting as recurrent episodes of vascular collapse: response to disodium cromoglycate and disease outcome.

Author

Conde-Fernandes I, Sampaio R, Moreno F, Palla-Garcia J, Teixeira MDA, Freitas I, Neves E, Jara-Acevedo M, Escribano L, and Lima M

Abstract

Background: Mastocytosis are rare diseases characterized by an accumulation of clonal mast cells (MCs) in one or multiple organs or tissues. Patients with systemic mastocytosis (SM), whose MCs frequently arbor the activating D816V KIT mutation, may have indolent to aggressive diseases, and they may experience MC mediator related symptoms. Indolent SM with recurrent anaphylaxis or vascular collapse in the absence of skin lesions, ISMs(-), is a specific subtype indolent SM (ISM), and this clonal MC activation disorder represents a significant fraction of all MC activation syndromes. The V560G KIT mutation is extremely rare in patients with SM and its biological and prognostic impact remains unknown., Case Presentation: A 15-year old boy was referred to our hospital because of repeated episodes of flushing, hypotension and syncope since the age of 3-years, preceded by skin lesions compatible with mastocytosis on histopathology that had disappeared in the late-early childhood. Diagnosis of ISM, more precisely the ISMs(-) variant, was confirmed based on the clinical manifestations together with increased baseline serum tryptase levels and the presence of morphologically atypical, mature appearing (CD117+high, FcεRI+) phenotypically aberrant (CD2+, CD25+) MCs, expressing activation-associated markers (CD63, CD69), in the bone marrow. Molecular genetic studies revealed the presence of the KIT V560G mutation in bone marrow MCs, but not in other bone marrow cells, whereas the screening for mutations in codon 816 of KIT was negative. The patient was treated with oral disodium cromoglycate and the disease had a favorable outcome after an eleven-year follow-up period, during which progressively lower serum tryptase levels together with the fully disappearance of all clinical manifestations was observed., Conclusions: To the best of our knowledge this first report of a patient with ISM, whose bone marrow MCs carry the KIT V560G activating mutation, manifesting as recurrent spontaneous episodes of flushing and vascular collapse in the absence of skin lesions at the time of diagnosis, in whom disodium cromoglycate had led to long term clinical remission.

Published

2017

41. A Next-Generation Sequencing Strategy for Evaluating the Most Common Genetic Abnormalities in Multiple Myeloma.

Author

Jiménez C, Jara-Acevedo M, Corchete LA, Castillo D, Ordóñez GR, Sarasquete ME, Puig N, Martínez-López J, Prieto-Conde MI, García-Álvarez M, Chillón MC, Balanzategui A, Alcoceba M, Oriol A, Rosiñol L, Palomera L, Teruel AI, Lahuerta JJ, Bladé J, Mateos MV, Orfão A, San Miguel JF, González M, Gutiérrez NC, and García-Sanz R

Subjects

Aged, Female, Gene Frequency, Genes, Neoplasm, Humans, Male, Middle Aged, Multiple Myeloma diagnosis, Mutation, DNA Mutational Analysis methods, High-Throughput Nucleotide Sequencing methods, Molecular Diagnostic Techniques, Multiple Myeloma genetics

Abstract

Identification and characterization of genetic alterations are essential for diagnosis of multiple myeloma and may guide therapeutic decisions. Currently, genomic analysis of myeloma to cover the diverse range of alterations with prognostic impact requires fluorescence in situ hybridization (FISH), single nucleotide polymorphism arrays, and sequencing techniques, which are costly and labor intensive and require large numbers of plasma cells. To overcome these limitations, we designed a targeted-capture next-generation sequencing approach for one-step identification of IGH translocations, V(D)J clonal rearrangements, the IgH isotype, and somatic mutations to rapidly identify risk groups and specific targetable molecular lesions. Forty-eight newly diagnosed myeloma patients were tested with the panel, which included IGH and six genes that are recurrently mutated in myeloma: NRAS, KRAS, HRAS, TP53, MYC, and BRAF. We identified 14 of 17 IGH translocations previously detected by FISH and three confirmed translocations not detected by FISH, with the additional advantage of breakpoint identification, which can be used as a target for evaluating minimal residual disease. IgH subclass and V(D)J rearrangements were identified in 77% and 65% of patients, respectively. Mutation analysis revealed the presence of missense protein-coding alterations in at least one of the evaluating genes in 16 of 48 patients (33%). This method may represent a time- and cost-effective diagnostic method for the molecular characterization of multiple myeloma., (Copyright © 2017 American Society for Investigative Pathology and the Association for Molecular Pathology. Published by Elsevier Inc. All rights reserved.)

Published

2017

42. Imatinib in systemic mastocytosis: a phase IV clinical trial in patients lacking exon 17 KIT mutations and review of the literature.

Author

Alvarez-Twose I, Matito A, Morgado JM, Sánchez-Muñoz L, Jara-Acevedo M, García-Montero A, Mayado A, Caldas C, Teodósio C, Muñoz-González JI, Mollejo M, Escribano L, and Orfao A

Abstract

Resistance to imatinib has been recurrently reported in systemic mastocytosis (SM) carrying exon 17 KIT mutations. We evaluated the efficacy and safety of imatinib therapy in 10 adult SM patients lacking exon 17 KIT mutations, 9 of which fulfilled criteria for well-differentiated SM (WDSM). The World Health Organization 2008 disease categories among WDSM patients were mast cell (MC) leukemia ( n = 3), indolent SM ( n = 3) and cutaneous mastocytosis ( n = 3); the remainder case had SM associated with a clonal haematological non-MC disease. Patients were given imatinib for 12 months -400 or 300 mg daily depending on the presence vs. absence of > 30% bone marrow (BM) MCs and/or signs of advanced disease-. Absence of exon 17 KIT mutations was confirmed in highly-purified BM MCs by peptide nucleic acid-mediated PCR, while mutations involving other exons were investigated by direct sequencing of purified BM MC DNA. Complete response (CR) was defined as resolution of BM MC infiltration, skin lesions, organomegalies and MC-mediator release-associated symptoms, plus normalization of serum tryptase. Criteria for partial response (PR) included ≥ 50% reduction in BM MC infiltration and improvement of skin lesions and/or organomegalies. Treatment was well-tolerated with an overall response rate of 50%, including early and sustained CR in four patients, three of whom had extracellular mutations of KIT , and PR in one case. This later patient and all non-responders ( n = 5) showed wild-type KIT . These results together with previous data from the literature support the relevance of the KIT mutational status in selecting SM patients who are candidates for imatinib therapy., Competing Interests: CONFLICTS OF INTEREST The authors declare no competing financial interest.

Published

2016

43. KIT D816V-mutated bone marrow mesenchymal stem cells in indolent systemic mastocytosis are associated with disease progression.

Author

Garcia-Montero AC, Jara-Acevedo M, Alvarez-Twose I, Teodosio C, Sanchez-Muñoz L, Muñiz C, Muñoz-Gonzalez JI, Mayado A, Matito A, Caldas C, Morgado JM, Escribano L, and Orfao A

Subjects

Adult, Aspartic Acid genetics, Bone Marrow Cells metabolism, Cell Lineage genetics, Disease Progression, Female, Humans, Immunophenotyping, Male, Mesenchymal Stem Cells metabolism, Mutation, Missense, Proto-Oncogene Proteins c-kit metabolism, Valine genetics, Amino Acid Substitution, Bone Marrow Cells pathology, Mastocytosis, Systemic genetics, Mastocytosis, Systemic pathology, Mesenchymal Stem Cells pathology, Proto-Oncogene Proteins c-kit genetics

Abstract

Multilineage involvement of bone marrow (BM) hematopoiesis by the somatic KIT D816V mutation is present in a subset of adult indolent systemic mastocytosis (ISM) patients in association with a poorer prognosis. Here, we investigated the potential involvement of BM mesenchymal stem cells (MSCs) from ISM patients by the KIT D816V mutation and its potential impact on disease progression and outcome. This mutation was investigated in highly purified BM MSCs and other BM cell populations from 83 ISM patients followed for a median of 116 months. KIT D816V-mutated MSCs were detected in 22 of 83 cases. All MSC-mutated patients had multilineage KIT mutation (100% vs 30%, P = .0001) and they more frequently showed involvement of lymphoid plus myeloid BM cells (59% vs 22%; P = .03) and a polyclonal pattern of inactivation of the X-chromosome of KIT-mutated BM mast cells (64% vs 0%; P = .01) vs other multilineage ISM cases. Moreover, presence of KIT-mutated MSCs was associated with more advanced disease features, a greater rate of disease progression (50% vs 17%; P = .04), and a shorter progression-free survival (P ≤ .003). Overall, these results support the notion that ISM patients with mutated MSCs may have acquired the KIT mutation in a common pluripotent progenitor cell, prior to differentiation into MSCs and hematopoietic precursor cells, before the X-chromosome inactivation process occurs. From a clinical point of view, acquisition of the KIT mutation in an earlier BM precursor cell confers a significantly greater risk for disease progression and a poorer outcome., (© 2016 by The American Society of Hematology.)

Published

2016

44. Clinical, immunophenotypic, and molecular characteristics of well-differentiated systemic mastocytosis.

Author

Álvarez-Twose I, Jara-Acevedo M, Morgado JM, García-Montero A, Sánchez-Muñoz L, Teodósio C, Matito A, Mayado A, Caldas C, Mollejo M, Orfao A, and Escribano L

Subjects

Adolescent, Adult, Aged, Child, Child, Preschool, Female, Humans, Immunophenotyping, Male, Mast Cells immunology, Mast Cells pathology, Mastocytosis, Cutaneous genetics, Mastocytosis, Cutaneous immunology, Mastocytosis, Cutaneous pathology, Mastocytosis, Systemic genetics, Mastocytosis, Systemic immunology, Mastocytosis, Systemic pathology, Middle Aged, Mutation, Proto-Oncogene Proteins c-kit genetics, Skin pathology, Young Adult, Mastocytosis, Cutaneous diagnosis, Mastocytosis, Systemic diagnosis

Abstract

Background: Well-differentiated systemic mastocytosis (WDSM) is a rare variant of systemic mastocytosis (SM) characterized by bone marrow (BM) infiltration by mature-appearing mast cells (MCs) often lacking exon 17 KIT mutations. Because of its rarity, the clinical and biological features of WDSM remain poorly defined., Objective: We sought to determine the clinical, biological, and molecular features of a cohort of 33 patients with mastocytosis in the skin in association with BM infiltration by well-differentiated MCs and to establish potential diagnostic criteria for WDSM., Methods: Thirty-three patients with mastocytosis in the skin plus BM aggregates of round, fully granulated MCs lacking strong CD25 and CD2 expression in association with clonal MC features were studied., Results: Our cohort of patients showed female predominance (female/male ratio, 4:1) and childhood onset of the disease (91%) with frequent familial aggregation (39%). Skin involvement was heterogeneous, including maculopapular (82%), nodular (6%), and diffuse cutaneous (12%) mastocytosis. KIT mutations were detected in only 10 (30%) of 33 patients, including the KIT D816V (n = 5), K509I (n = 3), N819Y (n = 1), and I817V (n = 1) mutations. BM MCs displayed a unique immunophenotypic pattern consisting of increased light scatter features, overexpression of cytoplasmic carboxypeptidase, and aberrant expression of CD30, together with absent (79%) or low (21%) positivity for CD25, CD2, or both. Despite only 9 (27%) of 33 patients fulfilling the World Health Organization criteria for SM, our findings allowed us to establish the systemic nature of the disease, which fit with the definition of WDSM., Conclusions: WDSM represents a rare clinically and molecularly heterogeneous variant of SM that requires unique diagnostic criteria to avoid a misdiagnosis of cutaneous mastocytosis per current World Health Organization criteria., (Copyright © 2015 American Academy of Allergy, Asthma & Immunology. Published by Elsevier Inc. All rights reserved.)

Published

2016

45. Diagnosis and classification of mastocytosis in non-specialized versus reference centres: a Spanish Network on Mastocytosis (REMA) study on 122 patients.

Author

Sánchez-Muñoz L, Morgado JM, Álvarez-Twose I, Matito A, Garcia-Montero AC, Teodosio C, Jara-Acevedo M, Mayado A, Mollejo M, Caldas C, González de Olano D, Escribano L, and Orfao A

Subjects

Adult, Aged, Aged, 80 and over, Bone Marrow pathology, Female, Humans, Immunophenotyping, Male, Mast Cells immunology, Mast Cells pathology, Mastocytosis classification, Mastocytosis genetics, Mastocytosis immunology, Middle Aged, Mutation, Proto-Oncogene Proteins c-kit genetics, Rare Diseases diagnosis, Referral and Consultation, Retrospective Studies, Spain, Specialization, Tryptases blood, Young Adult, Mastocytosis diagnosis

Abstract

The diagnosis of 'rare diseases', such as mastocytosis, remains a challenge. Despite this, the precise benefits of referral of mastocytosis patients to highly specialized reference centres are poorly defined and whether patients should be managed at non-specialized versus reference centres remains a matter of debate. To evaluate the quality and efficiency of diagnostic procedures performed at the reference centres for mastocytosis in Spain (REMA) versus other non-reference centres, we retrospectively analysed a series of 122 patients, for the overall degree of agreement obtained for the World Health Organization (WHO) diagnostic and classification criteria betwen the referring and REMA centres. Our results showed that not all WHO diagnostic criteria were frequently investigated at the referring centres. Among the five WHO diagnostic criteria, the highest degree of agreement was obtained for serum tryptase levels [median 90% (95% confidence interval 84-96%)]; in turn, the overall agreement was significantly lower for the major histopathological criterion [80% (72-89%)], and the other three minor criteria: cytomorphology [68% (56-80%)] immunophenotyping of BM mast cells [75% (62-87%)] and detection of the KIT mutation [34% (8-60%)]. Referral of patients with diagnostic suspicion of mastocytosis to a multidisciplinary reference centre improves diagnostic efficiency and quality., (© 2015 John Wiley & Sons Ltd.)

Published

2016

46. Phenotypic profile of expanded NK cells in chronic lymphoproliferative disorders: a surrogate marker for NK-cell clonality.

Author

Bárcena P, Jara-Acevedo M, Tabernero MD, López A, Sánchez ML, García-Montero AC, Muñoz-García N, Vidriales MB, Paiva A, Lecrevisse Q, Lima M, Langerak AW, Böttcher S, van Dongen JJ, Orfao A, and Almeida J

Subjects

Adult, Aged, Aged, 80 and over, Chronic Disease, Clone Cells pathology, Cluster Analysis, Female, Humans, Immunophenotyping, Middle Aged, Phenotype, Receptors, Androgen analysis, Biomarkers analysis, Flow Cytometry methods, Killer Cells, Natural pathology, Lymphoproliferative Disorders diagnosis

Abstract

Currently, the lack of a universal and specific marker of clonality hampers the diagnosis and classification of chronic expansions of natural killer (NK) cells. Here we investigated the utility of flow cytometric detection of aberrant/altered NK-cell phenotypes as a surrogate marker for clonality, in the diagnostic work-up of chronic lymphoproliferative disorders of NK cells (CLPD-NK). For this purpose, a large panel of markers was evaluated by multiparametric flow cytometry on peripheral blood (PB) CD56(low) NK cells from 60 patients, including 23 subjects with predefined clonal (n = 9) and polyclonal (n = 14) CD56(low) NK-cell expansions, and 37 with CLPD-NK of undetermined clonality; also, PB samples from 10 healthy adults were included. Clonality was established using the human androgen receptor (HUMARA) assay. Clonal NK cells were found to show decreased expression of CD7, CD11b and CD38, and higher CD2, CD94 and HLADR levels vs. normal NK cells, together with a restricted repertoire of expression of the CD158a, CD158b and CD161 killer-associated receptors. In turn, NK cells from both clonal and polyclonal CLPD-NK showed similar/overlapping phenotypic profiles, except for high and more homogeneous expression of CD94 and HLADR, which was restricted to clonal CLPD-NK. We conclude that the CD94(hi)/HLADR+ phenotypic profile proved to be a useful surrogate marker for NK-cell clonality.

Published

2015

47. Detection of the KIT D816V mutation in peripheral blood of systemic mastocytosis: diagnostic implications.

Author

Jara-Acevedo M, Teodosio C, Sanchez-Muñoz L, Álvarez-Twose I, Mayado A, Caldas C, Matito A, Morgado JM, Muñoz-González JI, Escribano L, Garcia-Montero AC, and Orfao A

Subjects

Bone Marrow Cells pathology, Bone Marrow Examination, Cell Lineage, Exons, Genetic Markers, Genetic Predisposition to Disease, Hematopoiesis genetics, Humans, Mast Cells pathology, Mastocytosis, Systemic blood, Phenotype, Predictive Value of Tests, Proto-Oncogene Proteins c-kit blood, Severity of Illness Index, Spain, DNA Mutational Analysis methods, Mastocytosis, Systemic diagnosis, Mastocytosis, Systemic genetics, Mutation, Polymerase Chain Reaction methods, Proto-Oncogene Proteins c-kit genetics

Abstract

Recent studies have found the KIT D816V mutation in peripheral blood of virtually all adult systemic mastocytosis patients once highly sensitive PCR techniques were used; thus, detection of the KIT D816V mutation in peripheral blood has been proposed to be included in the diagnostic work-up of systemic mastocytosis algorithms. However, the precise frequency of the mutation, the biological significance of peripheral blood-mutated cells and their potential association with involvement of bone marrow hematopoietic cells other than mast cells still remain to be investigated. Here, we determined the frequency of peripheral blood involvement by the KIT D816V mutation, as assessed by two highly sensitive PCR methods, and investigated its relationship with multilineage involvement of bone marrow hematopoiesis. Overall, our results confirmed the presence of the KIT D816V mutation in peripheral blood of most systemic mastocytosis cases (161/190; 85%)--with an increasing frequency from indolent systemic mastocytosis without skin lesions (29/44; 66%) to indolent systemic mastocytosis with skin involvement (124/135; 92%), and more aggressive disease subtypes (11/11; 100%)--as assessed by the allele-specific oligonucleotide-qPCR method, which was more sensitive (P<.0001) than the peptide nucleic acid-mediated PCR approach (84/190; 44%). Although the presence of the KIT mutation in peripheral blood, as assessed by the allele-specific oligonucleotide-qPCR technique, did not accurately predict for multilineage bone marrow involvement of hematopoiesis, the allele-specific oligonucleotide-qPCR allele burden and the peptide nucleic acid-mediated-PCR approach did. These results suggest that both methods provide clinically useful and complementary information through the identification and/or quantification of the KIT D816V mutation in peripheral blood of patients suspected of systemic mastocytosis.

Published

2015

48. The immunophenotype of mast cells and its utility in the diagnostic work-up of systemic mastocytosis.

Author

Teodosio C, Mayado A, Sánchez-Muñoz L, Morgado JM, Jara-Acevedo M, Álvarez-Twose I, García-Montero AC, Matito A, Caldas C, Escribano L, and Orfao A

Subjects

Animals, Humans, Mastocytosis, Systemic immunology, Immunophenotyping, Mast Cells immunology, Mastocytosis, Systemic diagnosis

Abstract

SM comprises a heterogeneous group of disorders, characterized by an abnormal accumulation of clonal MCs in 1 or more tissues, frequently involving the skin and BM. Despite the fact that most adult patients (>90%) carry the same genetic lesion (D816V KIT mutation), the disease presents with multiple variants with very distinct clinical and biologic features, a diverse prognosis, and different therapeutic requirements. Recent advances in the standardization of the study of BM MC by MFC allowed reproducible identification and characterization of normal/reactive MCs and their precursors, as well as the establishment of the normal MC maturational profiles. Analysis of large groups of patients versus normal/reactive samples has highlighted the existence of aberrant MC phenotypes in SM, which are essential for the diagnosis of the disease. In turn, 3 clearly distinct and altered maturation-associated immunophenotypic profiles have been reported recently in SM, which provide criteria for the distinction between ISM patients with MC-restricted and multilineage KIT mutation; thus, immunphenotyping also contributes to prognostic stratification of ISM, particularly when analysis of the KIT mutation on highly purified BM cells is not routinely available in the diagnostic work-up of the disease., (© Society for Leukocyte Biology.)

Published

2015

49. Flow cytometry in mastocytosis: utility as a diagnostic and prognostic tool.

Author

Sánchez-Muñoz L, Teodosio C, Morgado JM, Perbellini O, Mayado A, Alvarez-Twose I, Matito A, Jara-Acevedo M, García-Montero AC, Orfao A, and Escribano L

Subjects

Adult, Antigens, CD genetics, Antigens, CD immunology, Bone Marrow immunology, Flow Cytometry, Gene Expression, Humans, Immunophenotyping, Mast Cells immunology, Mastocytosis genetics, Mastocytosis immunology, Mastocytosis pathology, Mutation, Prognosis, Proto-Oncogene Proteins c-kit genetics, Proto-Oncogene Proteins c-kit immunology, Bone Marrow pathology, Mast Cells pathology, Mastocytosis diagnosis

Abstract

This article presents information for the identification and characterization of mast cells from bone marrow and other tissues using multiparametric flow cytometry. In addition, it provides guidelines for the application of this technique in the subclassification of systemic mastocytosis and assessment of the long-term prognosis of patients individually., (Copyright © 2014 Elsevier Inc. All rights reserved.)

Published

2014

50. Nonaggressive systemic mastocytosis (SM) without skin lesions associated with insect-induced anaphylaxis shows unique features versus other indolent SM.

Author

Alvarez-Twose I, Zanotti R, González-de-Olano D, Bonadonna P, Vega A, Matito A, Sánchez-Muñoz L, Morgado JM, Perbellini O, García-Montero A, De Matteis G, Teodósio C, Rossini M, Jara-Acevedo M, Schena D, Mayado A, Zamò A, Mollejo M, Sánchez-López P, Cabañes N, Orfao A, and Escribano L

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Allergens immunology, Anaphylaxis diagnosis, Animals, Female, Humans, Immunoglobulin E blood, Insect Bites and Stings diagnosis, Male, Mastocytosis, Systemic diagnosis, Middle Aged, Skin Diseases diagnosis, Skin Tests, Tryptases blood, Young Adult, Anaphylaxis immunology, Bees immunology, Insect Bites and Stings immunology, Mastocytosis, Systemic immunology, Skin Diseases immunology, Wasps immunology

Abstract

Background: Indolent systemic mastocytosis (ISM) without skin lesions (ISMs(-)) shows a higher prevalence in males, lower serum baseline tryptase levels, and KIT mutation more frequently restricted to bone marrow (BM) mast cells (MCs) than ISM with skin lesions (ISMs(+)). Interestingly, in almost one-half of ISMs(-) patients, MC-mediator release episodes are triggered exclusively by insects., Objective: We aimed to determine the clinical and laboratory features of ISMs(-) associated with insect-induced anaphylaxis (insectISMs(-)) versus other patients with ISM., Methods: A total of 335 patients presenting with MC activation syndrome, including 143 insectISMs(-), 72 ISMs(-) triggered by other factors (otherISMs(-)), 56 ISMs(+), and 64 nonclonal MC activation syndrome, were studied., Results: Compared with otherISMs(-) and ISMs(+) patients, insectISMs(-) cases showed marked male predominance (78% vs 53% and 46%; P < .001), a distinct pattern of MC-related symptoms, and significantly lower median serum baseline tryptase levels (22.4 vs 28.7 and 45.8 μg/L; P ≤ .009). Moreover, insectISMs(-) less frequently presented BM MC aggregates (46% vs 70% and 81%; P ≤ .001), and they systematically showed MC-restricted KIT mutation., Conclusions: ISMs(-) patients with anaphylaxis triggered exclusively by insects display clinical and laboratory features that are significantly different from other ISM cases, including other ISMs(-) and ISMs(+) patients, suggesting that they represent a unique subgroup of ISM with a particularly low BM MC burden in the absence of adverse prognostic factors., (Copyright © 2013 American Academy of Allergy, Asthma & Immunology. Published by Mosby, Inc. All rights reserved.)

Published

2014