Your search keyword '"van Dongen, J. J .M."' showing total 117 results

1. Automated EuroFlow approach for standardized in-depth dissection of human circulating B-cells and plasma cells.

Author

Delgado, Alejandro H., Fluxa, Rafael, Perez-Andres, Martin, Diks, Annieck M., van Gaans-van den Brink, Jacqueline A. M., Barkoff, Alex-Mikael, Blanco, Elena, Torres-Valle, Alba, Berkowska, Magdalena A., Grigore, Georgiana, van Dongen, J. J. M., and Orfao, Alberto

Subjects

PLASMA cells, HUMAN dissection, CORD blood, LYMPHOCYTE subsets, B cells

Abstract

Background: Multiparameter flow cytometry (FC) immunophenotyping is a key tool for detailed identification and characterization of human blood leucocytes, including B-lymphocytes and plasma cells (PC). However, currently used conventional data analysis strategies require extensive expertise, are time consuming, and show limited reproducibility. Objective: Here, we designed, constructed and validated an automated database-guided gating and identification (AGI) approach for fast and standardized in-depth dissection of B-lymphocyte and PC populations in human blood. Methods: For this purpose, 213 FC standard (FCS) datafiles corresponding to umbilical cord and peripheral blood samples from healthy and patient volunteers, stained with the 14-color 18-antibody EuroFlow BIgH-IMM panel, were used. Results: The BIgH-IMM antibody panel allowed identification of 117 different Blymphocyte and PC subsets. Samples from 36 healthy donors were stained and 14 of the datafiles that fulfilled strict inclusion criteria were analysed by an expert flow cytometrist to build the EuroFlow BIgH-IMM database. Data contained in the datafiles was then merged into a reference database that was uploaded in the Infinicyt software (Cytognos, Salamanca, Spain). Subsequently, we compared the results of manual gating (MG) with the performance of two classification algorithms -hierarchical algorithm vs two-step algorithm-for AGI of the cell populations present in 5 randomly selected FCS datafiles. The hierarchical AGI algorithm showed higher correlation values vs conventional MG (r2 of 0.94 vs. 0.88 for the two-step AGI algorithm) and was further validated in a set of 177 FCS datafiles against conventional expert-based MG. For virtually all identifiable cell populations a highly significant correlation was observed between the two approaches (r2>0.81 for 79% of all B-cell populations identified), with a significantly lower median time of analysis per sample (6 vs. 40 min, p=0.001) for the AGI tool vs. MG, respectively and both intra-sample (median CV of 1.7% vs. 10.4% by MG, p<0.001) and inter-expert (median CV of 3.9% vs. 17.3% by MG by 2 experts, p<0.001) variability. Conclusion: Our results show that compared to conventional FC data analysis strategies, the here proposed AGI tool is a faster, more robust, reproducible, and standardized approach for in-depth analysis of B-lymphocyte and PC subsets circulating in human blood. [ABSTRACT FROM AUTHOR]

Published

2023

2. IgE‐expressing memory B cells and plasmablasts are increased in blood of children with asthma, food allergy, and atopic dermatitis.

Author

Heeringa, J. J., Rijvers, L., Arends, N. J., Driessen, G. J., Pasmans, S. G., van Dongen, J. J. M., de Jongste, J. C., and van Zelm, M. C.

Subjects

IMMUNOGLOBULIN E, B cells, MEMORY, ASTHMA in children, FOOD allergy in children, ATOPIC dermatitis, BLOOD

Abstract

Abstract: Despite the critical role of soluble IgE in the pathology of IgE‐mediated allergic disease, little is known about abnormalities in the memory B cells and plasma cells that produce IgE in allergic patients. We here applied a flow cytometric approach to cross‐sectionally study blood IgE+ memory B cells and plasmablasts in 149 children with atopic dermatitis, food allergy, and/or asthma and correlated these to helper T(h)2 cells and eosinophils. Children with allergic disease had increased numbers of IgE+CD27‐ and IgE+CD27+ memory B cells and IgE+ plasmablasts, as well as increased numbers of eosinophils and Th2 cells. IgE+ plasmablast numbers correlated positively with Th2 cell numbers. These findings open new possibilities for diagnosis and monitoring of treatment in patients with allergic diseases. [ABSTRACT FROM AUTHOR]

Published

2018

3. Vorming en expressie van antigeenreceptoren op T- en B-lymfocyten.

Author

van Dongen, J. J. M., Langerak, A. W., and Kroese, F. G. M.

Published

2016

4. Basal Ca(2+) signaling is particularly increased in mutated chronic lymphocytic leukemia.

Author

Muggen, A F, Pillai, S Y, Kil, L P, van Zelm, M C, van Dongen, J J M, Hendriks, R W, and Langerak, A W

Abstract

On the basis of somatic hypermutation status of their B-cell antigen receptor (BCR) genes, chronic lymphocytic leukemia (CLL) patients can be divided into unmutated CLL (U-CLL) or mutated CLL (M-CLL). Approximately 30% of CLL patients express a stereotypic BCR, which may indicate that specific antigenic stimulation is driving CLL pathogenesis. Recently, it was reported that BCRs from CLL cells are capable of antigen-independent, cell-autonomous signaling, through recognition of an internal framework 2 (FR2) BCR epitope. We hypothesized that the level of cell-autonomous signaling may differ between CLL subgroups. Therefore, we analyzed Ca(2+) signaling in a series of primary stereotypic or heterogeneous U-CLL and M-CLL (n=68) and healthy controls (n=14). We confirmed that basal Ca(2+) signaling in CLL cells is higher than in normal B cells. Interestingly, we found that basal signaling was particularly increased in M-CLL. The degree of basal signaling did not correlate with membrane immunoglobulin levels, HCDR3 characteristics or FR2/FR3 sequence. We conclude that the level of basal Ca(2+) signaling is not uniformly enhanced in CLL B cells, but is associated with CLL immunoglobulin heavy chain V mutational status, reflecting a distinct cellular origin and possibly a different anergic state induced by repetitive or continuous antigen binding in vivo. [ABSTRACT FROM AUTHOR]

Published

2015

5. Basal Ca2+ signaling is particularly increased in mutated chronic lymphocytic leukemia.

Author

Muggen, A F, Pillai, S Y, Kil, L P, van Zelm, M C, van Dongen, J J M, Hendriks, R W, and Langerak, A W

Subjects

CHRONIC lymphocytic leukemia, ANTIGEN receptors, CARCINOGENESIS, IMMUNOGLOBULINS, EPITOPES

Abstract

On the basis of somatic hypermutation status of their B-cell antigen receptor (BCR) genes, chronic lymphocytic leukemia (CLL) patients can be divided into unmutated CLL (U-CLL) or mutated CLL (M-CLL). Approximately 30% of CLL patients express a stereotypic BCR, which may indicate that specific antigenic stimulation is driving CLL pathogenesis. Recently, it was reported that BCRs from CLL cells are capable of antigen-independent, cell-autonomous signaling, through recognition of an internal framework 2 (FR2) BCR epitope. We hypothesized that the level of cell-autonomous signaling may differ between CLL subgroups. Therefore, we analyzed Ca2+ signaling in a series of primary stereotypic or heterogeneous U-CLL and M-CLL (n=68) and healthy controls (n=14). We confirmed that basal Ca2+ signaling in CLL cells is higher than in normal B cells. Interestingly, we found that basal signaling was particularly increased in M-CLL. The degree of basal signaling did not correlate with membrane immunoglobulin levels, HCDR3 characteristics or FR2/FR3 sequence. We conclude that the level of basal Ca2+ signaling is not uniformly enhanced in CLL B cells, but is associated with CLL immunoglobulin heavy chain V mutational status, reflecting a distinct cellular origin and possibly a different anergic state induced by repetitive or continuous antigen binding in vivo. [ABSTRACT FROM AUTHOR]

Published

2015

6. 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, and San Miguel, J F

Subjects

MYELODYSPLASTIC syndromes, PLASMA cell diseases

Abstract

A letter to the editor is presented which discusses the examination of the presence of myelodysplastic syndrome (MDS)-associated phenotypic alterrations (MDS-PAs) in bone marrow (BM) samples from newly diagnosed patients referred immunophenotypic investigation of plasma cell (PC) neoplasia.

Published

2014

7. Persistent polyclonal B-cell lymphocytosis: extensively proliferated CD27+IgM+IgD+ memory B cells with a distinctive immunophenotype.

Author

Berkowska, M A, Grosserichter-Wagener, C, Adriaansen, H J, de Ridder, D, Mirani-Oostdijk, K P, Agteresch, H J, Böttcher, S, Orfao, A, van Dongen, J J M, and van Zelm, M C

Subjects

LYMPHOCYTOSIS, B cells, IMMUNOGLOBULIN M, IMMUNOGLOBULIN D, CELL proliferation, PATHOLOGICAL physiology

Abstract

The article discusses the nature of persistent polyclonal B-cell lymphocytosis (PPBL), a rare disease associated with smoking and mostly affects middle-aged women. It states that PPBL is characterized by persistent expansion of CD2+IgM+IgD+B cells, the increase IgM serum levels and the presence of circulating binucleated lymphocytes. It notes the extensive proliferation of such cells in PPBL. It also emphasizes the difference pathophysiology of the PPBL with mature B-cell malignancies.

Published

2014

8. Genetic and epigenetic determinants mediate proneness of oncogene breakpoint sites for involvement in TCR translocations.

Author

Larmonie, N S D, van der Spek, A, Bogers, A J J C, van Dongen, J J M, and Langerak, A W

Subjects

EPIGENETICS, DISEASE susceptibility, ONCOGENES, T cell receptors, LYMPHOBLASTIC leukemia, GENETIC recombination

Abstract

T-cell receptor (TCR) translocations are a genetic hallmark of T-cell acute lymphoblastic leukemia and lead to juxtaposition of oncogene and TCR loci. Oncogene loci become involved in translocations because they are accessible to the V(D)J recombination machinery. Such accessibility is predicted at cryptic recombination signal sequence (cRSS) sites ('Type 1') as well as other sites that are subject to DNA double-strand breaks (DSBs) ('Type 2') during early stages of thymocyte development. As chromatin accessibility markers have not been analyzed in the context of TCR-associated translocations, various genetic and epigenetic determinants of LMO2, TAL1 and TLX1 translocation breakpoint (BP) sites and BP cluster regions (BCRs) were examined in human thymocytes to establish DSB proneness and heterogeneity of BP site involvement in TCR translocations. Our data show that DSBs in BCRs are primarily induced in the presence of a genetic element of sequence vulnerability (cRSSs, transposable elements), whereas breaks at single BP sites lacking such elements are more likely induced by chance or perhaps because of patient-specific genetic vulnerability. Vulnerability to obtain DSBs is increased by features that determine chromatin organization, such as methylation status and nucleosome occupancy, although at different levels at different BP sites. [ABSTRACT FROM AUTHOR]

Published

2014

9. The clinical relevance of minor paroxysmal nocturnal hemoglobinuria clones in refractory cytopenia of childhood: a prospective study by EWOG-MDS.

Author

Aalbers, A M, van der Velden, V H J, Yoshimi, A, Fischer, A, Noellke, P, Zwaan, C M, Baumann, I, Beverloo, H B, Dworzak, M, Hasle, H, Locatelli, F, De Moerloose, B, Göhring, G, Schmugge, M, Stary, J, Zecca, M, Langerak, A W, van Dongen, J J M, Pieters, R, and Niemeyer, C M

Subjects

PAROXYSMAL hemoglobinuria, FLOW cytometry, IMMUNOSUPPRESSIVE agents, CLONE cells, LONGITUDINAL method

Abstract

The article presents a study which assesses the frequency of paroxysmal nocturnal hemoglobinuria (PNH) clones in refractory cytopenia of childhood (RCC) with high-sensitivity flow cytometry, and correlated the presence of PNH clones with clinical characteristics and response to immunosuppressive therapy (IST). It notes the attainment of peripheral blood samples for PNH analysis from 87 primary RCC patients. The study shows that PNH clones are frequently present in RCC.

Published

2014

10. The peripheral blood compartment in patients with Graves' disease: activated T lymphocytes and increased transitional and pre-naive mature B lymphocytes.

Author

Van der Weerd, K., Van Hagen, P. M., Schrijver, B., Kwekkeboom, D. J., De Herder, W. W., Ten Broek, M. R. J., Postema, P. T. E., Van Dongen, J. J. M., Staal, F. J. T., and Dik, W. A.

Subjects

GRAVES' disease, T cells, AUTOIMMUNE diseases, IMMUNOLOGICAL adjuvants, THYROID antagonists, FLOW cytometry, CD5 antigen

Abstract

Graves' disease ( GD) is an autoimmune disease that involves aberrant B and T lymphocyte responses. Detailed knowledge about lymphocyte subpopulation composition will therefore enhance our understanding of the pathogenesis of GD and might support the development of new immunomodulatory treatment approaches. The aim of this study was to gain detailed insight into the composition of the peripheral blood lymphocyte compartment in GD before and during anti-thyroid drug therapy. Major B and T lymphocyte subpopulations were investigated by flow cytometry in peripheral blood from newly diagnosed GD patients ( n = 5), GD patients treated with anti-thyroid drugs ( n = 4), patients with recurrent GD ( n = 7) and healthy controls ( HC; n = 10). In GD patients, numbers of activated T lymphocytes [human leucocyte antigen D-related ( HLA- DR)+ and CD25+] were increased. The B lymphocyte compartment in GD was characterized by significantly higher numbers of transitional ( CD38high CD27−, P < 0·03) and pre-naive mature ( CD38low CD27− IgD+ CD5+, P < 0·04) B lymphocytes, while memory populations were slightly decreased. The increased numbers of CD5+, transitional and pre-naive mature B lymphocytes correlated positively with fT4 plasma levels. GD is associated with increased numbers of activated T lymphocytes and transitional and pre-naive mature CD5+ B lymphocytes within the peripheral blood. The increase in CD5+ B lymphocytes was due mainly to an increase in transitional and pre-naive mature B lymphocytes. Increased fT4 plasma levels might be associated with this increase in transitional and pre-naive mature CD5+ B lymphocytes. [ABSTRACT FROM AUTHOR]

Published

2013

11. Improved flow cytometric detection of minimal residual disease in childhood acute lymphoblastic leukemia.

Author

Denys, B, van der Sluijs-Gelling, A J, Homburg, C, van der Schoot, C E, de Haas, V, Philippé, J, Pieters, R, van Dongen, J J M, and van der Velden, V H J

Subjects

LYMPHOBLASTIC leukemia in children, CYTOMETRY, BONE marrow, ANTIBODY formation, CELL cycle

Abstract

Most current treatment protocols for acute lymphoblastic leukemia (ALL) include minimal residual disease (MRD) diagnostics, generally based on PCR analysis of rearranged antigen receptor genes. Although flow cytometry (FCM) can be used for MRD detection as well, discordant FCM and PCR results are obtained in 5-20% of samples. We evaluated whether 6-color FCM, including additional markers and new marker combinations, improved the results. Bone marrow samples were obtained from 363 ALL patients at day 15, 33 and 78 and MRD was analyzed using 6-color (218 patients) or 4-color (145 patients) FCM in parallel to routine PCR-based MRD diagnostics. Compared with 4-color FCM, 6-color FCM significantly improved the concordance with PCR-based MRD data (88% versus 96%); particularly the specificity of the MRD analysis improved. However, PCR remained more sensitive at levels <0.01%. MRD-based risk groups were similar between 6-color FCM and PCR in 68% of patients, most discrepancies being medium risk by PCR and standard risk by FCM. Alternative interpretation of the PCR data, aimed at prevention of false-positive MRD results, changed the risk group to standard risk in half (52%) of these discordant cases. In conclusion, 6-color FCM significantly improves MRD analysis in ALL but remains less sensitive than PCR-based MRD-diagnostics. [ABSTRACT FROM AUTHOR]

Published

2013

12. EuroFlow standardization of flow cytometer instrument settings and immunophenotyping protocols.

Author

Kalina, T, Flores-Montero, J, van der Velden, V H J, Martin-Ayuso, M, Böttcher, S, Ritgen, M, Almeida, J, Lhermitte, L, Asnafi, V, Mendonça, A, de Tute, R, Cullen, M, Sedek, L, Vidriales, M B, Pérez, J J, te Marvelde, J G, Mejstrikova, E, Hrusak, O, Szczepański, T, and van Dongen, J J M

Subjects

FLOW cytometry, STANDARDIZATION, IMMUNOPHENOTYPING, HEMATOLOGICAL oncology, CANCER diagnosis

Abstract

The EU-supported EuroFlow Consortium aimed at innovation and standardization of immunophenotyping for diagnosis and classification of hematological malignancies by introducing 8-color flow cytometry with fully standardized laboratory procedures and antibody panels in order to achieve maximally comparable results among different laboratories. This required the selection of optimal combinations of compatible fluorochromes and the design and evaluation of adequate standard operating procedures (SOPs) for instrument setup, fluorescence compensation and sample preparation. Additionally, we developed software tools for the evaluation of individual antibody reagents and antibody panels. Each section describes what has been evaluated experimentally versus adopted based on existing data and experience. Multicentric evaluation demonstrated high levels of reproducibility based on strict implementation of the EuroFlow SOPs and antibody panels. Overall, the 6 years of extensive collaborative experiments and the analysis of hundreds of cell samples of patients and healthy controls in the EuroFlow centers have provided for the first time laboratory protocols and software tools for fully standardized 8-color flow cytometric immunophenotyping of normal and malignant leukocytes in bone marrow and blood; this has yielded highly comparable data sets, which can be integrated in a single database. [ABSTRACT FROM AUTHOR]

Published

2012

13. EuroFlow: Resetting leukemia and lymphoma immunophenotyping. Basis for companion diagnostics and personalized medicine.

Author

van Dongen, J J M and Orfao, A

Subjects

EDITORIALS, CONSORTIA, IMMUNOGLOBULINS, FLOW cytometry, MEDICAL software

Abstract

The authors reflect on the EuroFlow Consortium, which is supported by the European Union. They cite the main objectives of the project such as the development and testing of new antibodies, introduction of immunobead technology and flow cytometry software development. They state that the Consortium has achieved most of its goals with the development of an eight-color antibody protocols for hematological diagnosis.

Published

2012

14. EuroFlow antibody panels for standardized n-dimensional flow cytometric immunophenotyping of normal, reactive and malignant leukocytes.

Author

van Dongen, J J M, Lhermitte, L, Böttcher, S, Almeida, J, van der Velden, V H J, Flores-Montero, J, Rawstron, A, Asnafi, V, Lécrevisse, Q, Lucio, P, Mejstrikova, E, Szczepański, T, Kalina, T, de Tute, R, Brüggemann, M, Sedek, L, Cullen, M, Langerak, A W, Mendonça, A, and Macintyre, E

Subjects

IMMUNOPHENOTYPING, FLOW cytometry, HEMATOLOGIC malignancies, MULTIVARIATE analysis, CELL populations

Abstract

Most consensus leukemia & lymphoma antibody panels consist of lists of markers based on expert opinions, but they have not been validated. Here we present the validated EuroFlow 8-color antibody panels for immunophenotyping of hematological malignancies. The single-tube screening panels and multi-tube classification panels fit into the EuroFlow diagnostic algorithm with entries defined by clinical and laboratory parameters. The panels were constructed in 2-7 sequential design-evaluation-redesign rounds, using novel Infinicyt software tools for multivariate data analysis. Two groups of markers are combined in each 8-color tube: (i) backbone markers to identify distinct cell populations in a sample, and (ii) markers for characterization of specific cell populations. In multi-tube panels, the backbone markers were optimally placed at the same fluorochrome position in every tube, to provide identical multidimensional localization of the target cell population(s). The characterization markers were positioned according to the diagnostic utility of the combined markers. Each proposed antibody combination was tested against reference databases of normal and malignant cells from healthy subjects and WHO-based disease entities, respectively. The EuroFlow studies resulted in validated and flexible 8-color antibody panels for multidimensional identification and characterization of normal and aberrant cells, optimally suited for immunophenotypic screening and classification of hematological malignancies. [ABSTRACT FROM AUTHOR]

Published

2012

15. The EuroChimerism concept for a standardized approach to chimerism analysis after allogeneic stem cell transplantation.

Author

Lion, T, Watzinger, F, Preuner, S, Kreyenberg, H, Tilanus, M, de Weger, R, van Loon, J, de Vries, L, Cavé, H, Acquaviva, C, Lawler, M, Crampe, M, Serra, A, Saglio, B, Colnaghi, F, Biondi, A, van Dongen, J J M, van der Burg, M, Gonzalez, M, and Alcoceba, M

Subjects

CHIMERISM, STEM cell transplantation, POLYMERASE chain reaction, BIOLOGICAL assay, HEMATOPOIETIC stem cells

Abstract

Hematopoietic stem cell transplantation is becoming an increasingly important approach to treatment of different malignant and non-malignant disorders. There is thus growing demand for diagnostic assays permitting the surveillance of donor/recipient chimerism posttransplant. Current techniques are heterogeneous, rendering uniform evaluation and comparison of diagnostic results between centers difficult. Leading laboratories from 10 European countries have therefore performed a collaborative study supported by a European grant, the EuroChimerism Concerted Action, with the aim to develop a standardized diagnostic methodology for the detection and monitoring of chimerism in patients undergoing allogeneic stem cell transplantation. Following extensive analysis of a large set of microsatellite/short tandem repeat (STR) loci, the EuroChimerism (EUC) panel comprising 13 STR markers was established with the aim to optimally meet the specific requirements of quantitative chimerism analysis. Based on highly stringent selection criteria, the EUC panel provides multiple informative markers in any transplant setting. The standardized STR-PCR tests permit detection of donor- or recipient-derived cells at a sensitivity ranging between 0.8 and 1.6%. Moreover, the EUC assay facilitates accurate and reproducible quantification of donor and recipient hematopoietic cells. Wide use of the European-harmonized protocol for chimerism analysis presented will provide a basis for optimal diagnostic support and timely treatment decisions. [ABSTRACT FROM AUTHOR]

Published

2012

16. The novel calicheamicin-conjugated CD22 antibody inotuzumab ozogamicin (CMC-544) effectively kills primary pediatric acute lymphoblastic leukemia cells.

Author

de Vries, J F, Zwaan, C M, De Bie, M, Voerman, J S A, den Boer, M L, van Dongen, J J M, and van der Velden, V H J

Subjects

LYMPHOPROLIFERATIVE disorders, LYMPHOCYTIC leukemia, APOPTOSIS, ANEMIA, CELL death

Abstract

We investigated whether the newly developed antibody (Ab) -targeted therapy inotuzumab ozogamicin (CMC-544), consisting of a humanized CD22 Ab linked to calicheamicin, is effective in pediatric primary B-cell precursor acute lymphoblastic leukemia (BCP-ALL) cells in vitro, and analyzed which parameters determine its efficacy. CMC-544 induced dose-dependent cell kill in the majority of BCP-ALL cells, although IC50 values varied substantially (median 4.8 ng/ml, range 0.1-1000 ng/ml at 48 h). The efficacy of CMC-544 was highly dependent on calicheamicin sensitivity and CD22/CMC-544 internalization capacity of BCP-ALL cells, but hardly on basal and renewed CD22 expression. Although CD22 expression was essential for uptake of CMC-544, a repetitive loop of CD22 saturation, CD22/CMC-544 internalization and renewed CD22 expression was not required to achieve intracellular threshold levels of calicheamicin sufficient for efficient CMC-544-induced apoptosis in BCP-ALL cells. This is in contrast to studies with the comparable CD33 immunotoxin gemtuzumab ozogamicin (Mylotarg) in acute myeloid leukemia (AML) patients, in which complete and prolonged CD33 saturation was required for apoptosis induction. These data suggest that CMC-544 treatment may result in higher response rates in ALL compared with response rates obtained in AML with Mylotarg, and that therefore clinical studies in ALL, preferably with multiple low CMC-544 dosages, are warranted. [ABSTRACT FROM AUTHOR]

Published

2012

17. Correction of murine Rag1 deficiency by self-inactivating lentiviral vector-mediated gene transfer.

Author

Pike-Overzet, K., Rodijk, M., Ng, Y.-Y., Baert, M. R. M., Lagresle-Peyrou, C., Schambach, A., Zhang, F., Hoeben, R. C., Hacein-Bey-Abina, S., Lankester, A. C., Bredius, R. G. M., Driessen, G. J. A., Thrasher, A. J., Baum, C., Cavazzana-Calvo, M., van Dongen, J. J. M., and Staal, F. J. T.

Subjects

SEVERE combined immunodeficiency, CYTOKINES, MUTAGENESIS, GENETIC transformation, GENE therapy, T cell receptors, BONE marrow transplantation, B cells, T cells, ANIMAL experimentation, BONE marrow, CELL physiology, CELL receptors, COMPARATIVE studies, ENZYME-linked immunosorbent assay, FLOW cytometry, GENES, GENETIC techniques, IMMUNOGLOBULINS, RESEARCH methodology, MEDICAL cooperation, MICE, POLYMERASE chain reaction, PROTEINS, RESEARCH, RESEARCH funding, RETROVIRUSES, RNA, SPLEEN, WESTERN immunoblotting, EVALUATION research, REVERSE transcriptase polymerase chain reaction, THERAPEUTICS, PHYSIOLOGY

Abstract

Severe combined immunodeficiency (SCID) patients with an inactivating mutation in recombination activation gene 1 (RAG1) lack B and T cells due to the inability to rearrange immunoglobulin (Ig) and T-cell receptor (TCR) genes. Gene therapy is a valid treatment option for RAG-SCID patients, especially for patients lacking a suitable bone marrow donor, but developing such therapy has proven challenging. As a preclinical model for RAG-SCID, we used Rag1-/- mice and lentiviral self-inactivating (SIN) vectors harboring different internal elements to deliver native or codon-optimized human RAG1 sequences. Treatment resulted in the appearance of B and T cells in peripheral blood and developing B and T cells were detected in central lymphoid organs. Serum Ig levels and Ig and TCR Vβ gene segment usage was comparable to wild-type (WT) controls, indicating that RAG-mediated rearrangement took place. Remarkably, relatively low frequencies of B cells produced WT levels of serum immunoglobulins. Upon stimulation of the TCR, corrected spleen cells proliferated and produced cytokines. In vivo challenge resulted in production of antigen-specific antibodies. No leukemia development as consequence of insertional mutagenesis was observed. The functional reconstitution of the B- as well as the T-cell compartment provides proof-of-principle for therapeutic RAG1 gene transfer in Rag1-/- mice using lentiviral SIN vectors. [ABSTRACT FROM AUTHOR]

Published

2011

18. Standardization of DNA isolation from low cell numbers for chimerism analysis by PCR of short tandem repeats.

Author

Van der Burg, M., Kreyenberg, H., Willasch, A., Barendregt, B. H., Preuner, S., Watzinger, F., Lion, T., Roosnek, E., Harvey, J., Alcoceba, M., Díaz, M. G., Bader, P., and Van Dongen, J. J. M.

Subjects

CHIMERISM, STEM cell transplantation, POLYMERASE chain reaction, PROTOCOL analysis (Cognition)

Abstract

Analysis of short tandem repeats (STR) by PCR analysis is routinely used in chimerism diagnostics to monitor donor engraftment and to diagnose relapse. Some applications require chimerism analysis of low cell numbers, but no standardized protocol is available for DNA isolation from 1000 to 30 000 cells. The EU-supported EuroChimerism Consortium (project QLRT-2001-01485) selected four different protocols for 'small-scale' DNA isolation, which were tested by six laboratories for their ability to recover reproducible amounts of good quality DNA, suited for PCR-based STR analysis. The protocols included two direct lysis methods with and without detergents and proteinase K, and two commercial column-based kits. The direct lysis method using detergents and proteinase K showed the highest DNA recovery and the best performance in the multiplex PowerPlex16 STR assay. DNA isolated with this method also showed the highest sensitivity in chimerism analysis using singleplex PCR reactions of EuroChimerism STR markers. Sensitivity was reached ranging from 1 to 20% of recipient cells in a donor background. In conclusion, the direct lysis method using detergents and proteinase K is a standardized DNA isolation method well suited for chimerism studies on low cell numbers. [ABSTRACT FROM AUTHOR]

Published

2011

19. Artemis splice defects cause atypical SCID and can be restored in vitro by an antisense oligonucleotide.

Author

IJspeert, H, Lankester, A C, van den Berg, J M, Wiegant, W, van Zelm, M C, Weemaes, C M R, Warris, A, Pan-Hammarström, Q, Pastink, A, van Tol, M J D, van Dongen, J J M, van Gent, D C, and van der Burg, M

Subjects

SEVERE combined immunodeficiency, ANTISENSE nucleic acids, OLIGONUCLEOTIDES, GENETIC mutation, STEM cell transplantation, IONIZING radiation, IMMUNOGLOBULINS

Abstract

Artemis deficiency is known to result in classical T−B− severe combined immunodeficiency (SCID) in case of Artemis null mutations, or Omenn's syndrome in case of hypomorphic mutations in the Artemis gene. We describe two unrelated patients with a relatively mild clinical T−B− SCID phenotype, caused by different homozygous Artemis splice-site mutations. The splice-site mutations concern either dysfunction of a 5′ splice-site or an intronic point mutation creating a novel 3′ splice-site, resulting in mutated Artemis protein with residual activity or low levels of wild type (WT) Artemis transcripts. During the first 10 years of life, the patients suffered from recurrent infections necessitating antibiotic prophylaxis and intravenous immunoglobulins. Both mutations resulted in increased ionizing radiation sensitivity and insufficient variable, diversity and joining (V(D)J) recombination, causing B-lymphopenia and exhaustion of the naive T-cell compartment. The patient with the novel 3′ splice-site had progressive granulomatous skin lesions, which disappeared after stem cell transplantation (SCT). We showed that an alternative approach to SCT can, in principle, be used in this case; an antisense oligonucleotide (AON) covering the intronic mutation restored WT Artemis transcript levels and non-homologous end-joining pathway activity in the patient fibroblasts. [ABSTRACT FROM AUTHOR]

Published

2011

20. Integrated use of minimal residual disease classification and IKZF1 alteration status accurately predicts 79% of relapses in pediatric acute lymphoblastic leukemia.

Author

Waanders, E., van der Velden, V. H. J., van der Schoot, C. E., van Leeuwen, F. N., van Reijmersdal, S. V., de Haas, V., Veerman, A. J., van Kessel, A. Geurts, Hoogerbrugge, P. M., Kuiper, R. P., and van Dongen, J. J. M.

Subjects

LYMPHOBLASTIC leukemia in children, DISEASE relapse, ZINC-finger proteins, IMMUNOSPECIFICITY, PEDIATRIC therapy, LEUKEMIA

Abstract

Response to therapy as determined by minimal residual disease (MRD) is currently used for stratification in treatment protocols for pediatric acute lymphoblastic leukemia (ALL). However, the large MRD-based medium risk group (MRD-M; 50-60% of the patients) harbors many relapses. We analyzed MRD in 131 uniformly treated precursor-B-ALL patients and evaluated whether combined MRD and IKZF1 (Ikaros zinc finger-1) alteration status can improve risk stratification. We confirmed the strong prognostic significance of MRD classification, which was independent of IKZF1 alterations. Notably, 8 of the 11 relapsed cases in the large MRD-M group (n=81; 62%) harbored an IKZF1 alteration. Integration of both MRD and IKZF1 status resulted in a favorable outcome group (n=104; 5 relapses) and a poor outcome group (n=27; 19 relapses), and showed a stronger prognostic value than each of the established risk factors alone (hazard ratio (95%CI): 24.98 (8.29-75.31)). Importantly, whereas MRD and IKZF1 status alone identified only 46 and 54% of the relapses, respectively, their integrated use allowed prediction of 79% of all the relapses with 93% specificity. Because of the unprecedented sensitivity in upfront relapse prediction, the combined parameters have high potential for future risk stratification, particularly for patients originally classified as non-high risk, such as the large group of MRD-M patients. [ABSTRACT FROM AUTHOR]

Published

2011

21. Automated pattern-guided principal component analysis vs expert-based immunophenotypic classification of B-cell chronic lymphoproliferative disorders: a step forward in the standardization of clinical immunophenotyping.

Author

Costa, E. S., Pedreira, C. E., Barrena, S., Lecrevisse, Q., Flores, J., Quijano, S., Almeida, J., del Carmen García- Macias, M., Bottcher, S., Van Dongen, J. J. M., Orfao, A., and del Carmen García-Macias, M

Subjects

LYMPHATIC diseases, LYMPHOCYTIC leukemia, LYMPHOMAS, PUBLIC health

Abstract

Immunophenotypic characterization of B-cell chronic lymphoproliferative disorders (B-CLPD) is becoming increasingly complex due to usage of progressively larger panels of reagents and a high number of World Health Organization (WHO) entities. Typically, data analysis is performed separately for each stained aliquot of a sample; subsequently, an expert interprets the overall immunophenotypic profile (IP) of neoplastic B-cells and assigns it to specific diagnostic categories. We constructed a principal component analysis (PCA)-based tool to guide immunophenotypic classification of B-CLPD. Three reference groups of immunophenotypic data files-B-cell chronic lymphocytic leukemias (B-CLL; n = 10), mantle cell (MCL; n = 10) and follicular lymphomas (FL; n = 10)--were built. Subsequently, each of the 175 cases studied was evaluated and assigned to either one of the three reference groups or to none of them (other B-CLPD). Most cases (89%) were correctly assigned to their corresponding WHO diagnostic group with overall positive and negative predictive values of 89 and 96%, respectively. The efficiency of the PCA-based approach was particularly high among typical B-CLL, MCL and FL vs other B-CLPD cases. In summary, PCA-guided immunophenotypic classification of B-CLPD is a promising tool for standardized interpretation of tumor IP, their classification into well-defined entities and comprehensive evaluation of antibody panels. [ABSTRACT FROM AUTHOR]

Published

2010

22. B-cell maturation and antibody responses in individuals carrying a mutated CD19 allele.

Author

Artac, H., Reisli, I., Kara, R., Pico-Knijnenburg, I., Adin-Çinar, S., Pekcan, S., Jol-van der Zijde, C. M., van Tol, M. J. D., Bakker-Jonges, L. E., van Dongen, J. J. M., van der Burg, M., and van Zelm, M. C.

Subjects

B cell differentiation, CD antigens, GENETIC mutation, PERIPHERAL circulation, ANTIGEN-antibody reactions

Abstract

Homozygous CD19 mutations lead to an antibody deficiency due to disruption of the CD19 complex and consequent impaired signaling by the B-cell antigen receptor. We studied the effects of heterozygous CD19 mutations on peripheral B-cell development and antibody responses in a large family with multiple consanguineous marriages. Sequence analysis of 96 family members revealed 30 carriers of the CD19 mutation. Lymphocyte subset counts were not significantly different between carriers and noncarriers in three different age groups (0-10 years; 11-18 years; adults). B cells of carriers had reduced CD19 and CD21 median expression levels, and had reduced proportions of transitional (0-10 years) and CD5+ B cells (adults). CD19 carriers did not show clinical signs of immunodeficiency; they were well capable to produce normal serum Ig levels and had normal responses to primary and booster vaccinations. The frequency of mutated Vκ alleles was not affected. Heterozygous loss of CD19 causes some changes in the naive B-cell compartment, but overall in vivo B-cell maturation or humoral immunity is not affected. Many antibody deficiencies are not monogenetic, but likely caused by a combination of multiple genetic variations. Therefore, functional analyses of immune cell function should be carried out to show whether heterozygous mutations contribute to disease. [ABSTRACT FROM AUTHOR]

Published

2010

23. Clinical significance of flowcytometric minimal residual disease detection in pediatric acute myeloid leukemia patients treated according to the DCOG ANLL97/MRC AML12 protocol.

Author

van der Velden, V. H. J., van der Sluijs-Geling, A., Gibson, B. E. S., te Marvelde, J. G., Hoogeveen, P. G., Hop, W. C. J., Wheatley, K., Bierings, M. B., Schuurhuis, G. J., de Graaf, S. S. N., van Wering, E. R., and van Dongen, J. J. M.

Subjects

ACUTE myeloid leukemia in children, LEUKEMIA, CANCER treatment, DRUG therapy, MULTIVARIATE analysis, PATIENTS

Abstract

Analysis of minimal residual disease (MRD) in childhood acute myeloid leukemia (AML) may predict for clinical outcome. MRD levels were assessed by flowcytometric immunophenotyping in 94 children with AML enrolled into a single trial (United Kingdom Medical Research Council AML12 and similar Dutch Childhood Oncology Group ANLL97). An aberrant immunophenotype could be detected in 94% of patients. MRD levels after the first course of chemotherapy predicted for clinical outcome: 3-year relapse-free survival was 85%+/-8% (s.e.) for MRD-negative patients (MRD<0.1%), 64%+/-10% for MRD-low-positive patients (0.1%or=0.5%; P<0.001), whereas overall survival was 95%+/-5%, 70%+/-10% and 40%+/-13%, respectively, (P<0.001). Multivariate analysis allowing for age, karyotype, FLT3-internal tandem duplications and white blood cell count at diagnosis showed that MRD after the first course of chemotherapy was an independent prognostic factor. Although comparison of paired diagnosis-relapse samples (n=23) showed immunophenotypic shifts in 91% of cases, this did not hamper MRD analysis. In conclusion, flowcytometric MRD detection is possible in children with AML. The level of MRD after the first course of chemotherapy provides prognostic information that may be used to guide therapy. [ABSTRACT FROM AUTHOR]

Published

2010

24. Correction of B-cell development in Btk-deficient mice using lentiviral vectors with codon-optimized human BTK.

Author

Ng, Y. Y., Baert, M. R. M., Pike-Overzet, K., Rodijk, M., Brugman, M. H., Schambach, A., Baum, C., Hendriks, R. W., van Dongen, J. J. M., and Staal, F. J. T.

Subjects

AGAMMAGLOBULINEMIA, LYMPHOPROLIFERATIVE disorders, IMMUNOLOGICAL deficiency syndromes, GENES, CELL division, GENETIC engineering, IMMUNOGLOBULINS, LABORATORY mice

Abstract

X-linked agammaglobulinemia (XLA) is the most common primary immunodeficiency (PID) in man and caused by mutations in the Bruton’s tyrosine kinase (BTK) gene. XLA is characterized by a B-cell differentiation arrest in bone marrow, absence of mature B cells and immunoglobulins (Igs), and recurrent bacterial infections. We used self-inactivating lentiviral vectors expressing codon-optimized human BTK under the control of three different ubiquitous or B cell-specific promoters. Btk−/− mice engrafted with transduced cells showed correction of both precursor B-cell and peripheral B-cell development. Lentiviral vectors containing the wildtype BTK sequence did not correct the phenotype. All treated mice with codon-optimized BTK exhibited the recovery of B1 cells in the peritoneal cavity, and of serum IgM and IgG3 levels. Calcium mobilization responses upon B-cell receptor stimulation as well as in vivo responses to T cell-independent antigens were restored. Viral promoters overexpressing BTK >100-fold above normal resulted in erythro-myeloid proliferations independent of insertional mutagenesis. However, transplantation into secondary Btk−/− recipients using cellular promoters resulted in functional restoration of peripheral B cells and IgM levels, without any adverse effects. In conclusion, transduction of human BTK corrects B-cell development and antigen-specific antibody responses in Btk−/− mice, thus indicating the feasibility of lentiviral gene therapy for XLA, provided that BTK expression does not vastly exceed normal levels. [ABSTRACT FROM AUTHOR]

Published

2010

25. Preemptive alloimmune intervention in high-risk pediatric acute lymphoblastic leukemia patients guided by minimal residual disease level before stem cell transplantation.

Author

Lankester, A. C., Bierings, M. B., van Wering, E. R., Wijkhuijs, A. J. M., de Weger, R. A., Wijnen, J. T., Vossen, J. M., Versluys, B., Egeler, R. M., van Tol, M. J. D., Putter, H., Révész, T., van Dongen, J. J. M., van der Velden, V. H. J., and Schilham, M. W.

Subjects

LYMPHOCYTIC leukemia, STEM cell transplantation, CHILDHOOD cancer, CANCER patients, CYCLOSPORINE

Abstract

Relapse of pediatric acute lymphoblastic leukemia (ALL) remains the main cause of treatment failure after allogeneic stem cell transplantation (alloSCT). A high level of minimal residual disease (MRD) before alloSCT has been shown to predict these relapses. Patients at risk might benefit from a preemptive alloimmune intervention. In this first prospective, MRD-guided intervention study, 48 patients were stratified according to pre-SCT MRD level. Eighteen children with MRD level 1 × 10−4 were eligible for intervention, consisting of early cyclosporine A tapering followed by consecutive, incremental donor lymphocyte infusions (n=1–4). The intervention was associated with graft versus host disease grade II in only 23% of patients. Event-free survival in the intervention group was 19%. However, in contrast with the usual early recurrence of leukemia, relapses were delayed up to 3 years after SCT. In addition, several relapses presented at unusual extramedullary sites suggesting that the immune intervention may have altered the pattern of leukemia recurrence. In 8 out of 11 evaluable patients, relapse was preceded by MRD recurrence (median 9 weeks, range 0–30). We conclude that in children with high-risk ALL, immunotherapy-based regimens after SCT are feasible and may need to be further intensified to achieve total eradication of residual leukemic cells. [ABSTRACT FROM AUTHOR]

Published

2010

26. IKZF1 deletions predict relapse in uniformly treated pediatric precursor B-ALL.

Author

Kuiper, R. P., Waanders, E., van der Velden, V. H. J., van Reijmersdal, S. V., Venkatachalam, R., Scheijen, B., Sonneveld, E., van Dongen, J. J. M., Veerman, A. J. P., van Leeuwen, F. N., Geurts van Kessel, A., and Hoogerbrugge, P. M.

Subjects

LYMPHOBLASTIC leukemia, DISEASE complications, DNA, GENETIC mutation, HUMAN abnormalities

Abstract

Relapse is the most common cause of treatment failure in pediatric acute lymphoblastic leukemia (ALL) and is often difficult to predict. To explore the prognostic impact of recurrent DNA copy number abnormalities on relapse, we performed high-resolution genomic profiling of 34 paired diagnosis and relapse ALL samples. Recurrent lesions detected at diagnosis, including PAX5, CDKN2A and EBF1, were frequently absent at relapse, indicating that they represent secondary events that may be absent in the relapse-prone therapy-resistant progenitor cell. In contrast, deletions and nonsense mutations in IKZF1 (IKAROS) were highly enriched and consistently preserved at the time of relapse. A targeted copy number screen in an unselected cohort of 131 precursor B-ALL cases, enrolled in the dexamethasone-based Dutch Childhood Oncology Group treatment protocol ALL9, revealed that IKZF1 deletions are significantly associated with poor relapse-free and overall survival rates. Separate analysis of ALL9-treatment subgroups revealed that non-high-risk (NHR) patients with IKZF1 deletions exhibited a ∼12-fold higher relative relapse rate than those without IKZF1 deletions. Consequently, IKZF1 deletion status allowed the prospective identification of 53% of the relapse-prone NHR-classified patients within this subgroup and, therefore, serves as one of the strongest predictors of relapse at the time of diagnosis with high potential for future risk stratification. [ABSTRACT FROM AUTHOR]

Published

2010

27. Bimodal distribution of genomic MLL breakpoints in infant acute lymphoblastic leukemia treatment.

Author

Jung, R., Jacobs, U., Krumbholz, M., Langer, T., Keller, T., De Lorenzo, P., Valsecchi, M. G., van der Velden, V. H. J., Moericke, A., Stanulla, M., Teigler-Schlegel, A., Panzer-Gruemayer, E. R., van Dongen, J. J. M., Schrappe, M., den Boer, M. L., Pieters, R., Rascher, W., and Metzler, M.

Subjects

LETTERS to the editor, LYMPHOBLASTIC leukemia

Abstract

A letter to the editor is presented related to the treatment of acute lymphoblastic leukemia in children.

Published

2010

28. Genome-wide expression analysis of paired diagnosis–relapse samples in ALL indicates involvement of pathways related to DNA replication, cell cycle and DNA repair, independent of immune phenotype.

Author

Staal, F J T, de Ridder, D, Szczepanski, T, Schonewille, T, van der Linden, E C E, van Wering, E R, van der Velden, V H J, and van Dongen, J J M

Subjects

LYMPHOBLASTIC leukemia, PEDIATRICS, CANCER relapse, JUVENILE diseases, B cells, CANCER genes, GENE expression

Abstract

Almost a quarter of pediatric patients with acute lymphoblastic leukemia (ALL) suffer from relapses. The biological mechanisms underlying therapy response and development of relapses have remained unclear. In an attempt to better understand this phenomenon, we have analyzed 41 matched diagnosis–relapse pairs of ALL patients using genome-wide expression arrays (82 arrays) on purified leukemic cells. In roughly half of the patients, very few differences between diagnosis and relapse samples were found (‘stable group’), suggesting that mostly extra-leukemic factors (for example, drug distribution, drug metabolism, compliance) contributed to the relapse. Therefore, we focused our further analysis on 20 sample pairs with clear differences in gene expression (‘skewed group’), reasoning that these would allow us to better study the biological mechanisms underlying relapsed ALL. After finding the differences between diagnosis and relapse pairs in this group, we identified four major gene clusters corresponding to several pathways associated with changes in cell cycle, DNA replication, recombination and repair, as well as B-cell developmental genes. We also identified cancer genes commonly associated with colon carcinomas and ubiquitination to be upregulated in relapsed ALL. Thus, about half of the relapses are due to the selection or emergence of a clone with deregulated expression of genes involved in pathways that regulate B-cell signaling, development, cell cycle, cellular division and replication. [ABSTRACT FROM AUTHOR]

Published

2010

29. New insights to the MLL recombinome of acute leukemias.

Author

Meyer, C., Kowarz, E., Hofmann, J., Renneville, A., Zuna, J., Trka, J., Abdelali, R. Ben, Macintyre, E., De Braekeleer, E., De Braekeleer, M., Delabesse, E., de Oliveira, M. P., Cavé, H., Clappier, E., van Dongen, J. J. M., Balgobind, B. V., van den Heuvel-Eibrink, M. M., Beverloo, H. B., Panzer-Grümayer, R., and Teigler-Schlegel, A.

Subjects

LEUKEMIA, LYMPHOBLASTIC leukemia, CANCER treatment, GENOMES, PEDIATRICS

Abstract

Chromosomal rearrangements of the human MLL gene are associated with high-risk pediatric, adult and therapy-associated acute leukemias. These patients need to be identified, treated appropriately and minimal residual disease was monitored by quantitative PCR techniques. Genomic DNA was isolated from individual acute leukemia patients to identify and characterize chromosomal rearrangements involving the human MLL gene. A total of 760 MLL-rearranged biopsy samples obtained from 384 pediatric and 376 adult leukemia patients were characterized at the molecular level. The distribution of MLL breakpoints for clinical subtypes (acute lymphoblastic leukemia, acute myeloid leukemia, pediatric and adult) and fused translocation partner genes (TPGs) will be presented, including novel MLL fusion genes. Combined data of our study and recently published data revealed 104 different MLL rearrangements of which 64 TPGs are now characterized on the molecular level. Nine TPGs seem to be predominantly involved in genetic recombinations of MLL: AFF1/AF4, MLLT3/AF9, MLLT1/ENL, MLLT10/AF10, MLLT4/AF6, ELL, EPS15/AF1P, MLLT6/AF17 and SEPT6, respectively. Moreover, we describe for the first time the genetic network of reciprocal MLL gene fusions deriving from complex rearrangements. [ABSTRACT FROM AUTHOR]

Published

2009

30. Prognostic significance of minimal residual disease in infants with acute lymphoblastic leukemia treated within the Interfant-99 protocol.

Author

Van der Velden, V. H. J., Corral, L., Valsecchi, M. G., Jansen, M. W. J. C., De Lorenzo, P., Cazzaniga, G., Panzer-Grümayer, E. R., Schrappe, M., Schrauder, A., Meyer, C., Marschalek, R., Nigro, L. L., Metzler, M., Basso, G., Mann, G., Den Boer, M. L., Biondi, A., Pieters, R., Van Dongen, J. J. M., and Panzer-Grümayer, E R

Subjects

INFANT diseases, LYMPHOBLASTIC leukemia, T-cell receptor genes, BINDING sites, CELL membranes, LYMPHOBLASTIC leukemia diagnosis, THERAPEUTIC use of antineoplastic agents, PROTEINS, RESEARCH, CLINICAL trials, CARCINOGENESIS, RESEARCH methodology, CELL receptors, PROGNOSIS, EVALUATION research, MEDICAL cooperation, DISEASE relapse, TREATMENT effectiveness, COMPARATIVE studies, TRANSFERASES, GENES, RESEARCH funding, POLYMERASE chain reaction, LONGITUDINAL method

Abstract

Acute lymphoblastic leukemia (ALL) in infants younger than 1 year is a rare but relatively homogeneous disease ( approximately 80% MLL gene rearranged, approximately 70% CD10-negative) when compared with childhood and adult ALL. Several studies in children and adults with ALL have shown that minimal residual disease (MRD) status is a strong and independent prognostic factor. We therefore evaluated the prognostic significance of MRD in infant ALL. Ninety-nine infant patients treated according to the Interfant-99 protocol were included in this study. MRD was analyzed by real-time quantitative PCR analysis of rearranged immunoglobulin genes, T-cell receptor genes and MLL genes at various time points (TP) during therapy. Higher MRD levels at the end of induction (TP2) and consolidation (TP3) were significantly associated with lower disease-free survival. Combined MRD information at TP2 and TP3 allowed recognition of three patients groups that significantly differed in outcome. All MRD-high-risk patients (MRD levels > or =10(-4) at TP3; 26% of patients) relapsed. MRD-low-risk patients (MRD level <10(-4) at both TP2 and TP3) constituted 44% of patients and showed a relapse-rate of only 13%, whereas remaining patients (MRD-medium-risk patients; 30% of patients) had a relapse rate of 31%. Comparison between the current Interfant-06 stratification at diagnosis and the here presented MRD-based stratification showed that both stratifications recognized different subgroups of patients. These data indicate that MRD diagnostics has added value for recognition of risk groups in infant ALL and that MRD diagnostics can be used for treatment intervention in infant ALL as well. [ABSTRACT FROM AUTHOR]

Published

2009

31. Chromosome 14 copy number-dependent IGH gene rearrangement patterns in high hyperdiploid childhood B-cell precursor ALL: implications for leukemia biology and minimal residual disease analysis.

Author

Csinady, E., Van der Velden, V. H. J., Joas, R., Fischer, S., de Vries, J. F., Beverloo, H. B., König, M., Pötschger, U., Van Dongen, J. J. M., Mann, G., Haas, O. A., and Panzer-Grümayer, E. R.

Subjects

LYMPHOBLASTIC leukemia, MONOCLONAL antibodies, B cells, T cell receptors, HUMAN cytogenetics, GENDER mainstreaming

Abstract

Childhood B-cell precursor acute lymphoblastic leukemia (BCP ALL) is generally a clonal disease in which the number of IGH rearrangements per cell does not exceed the number of the IGH alleles on chromosome 14. Consequently, monoclonal high hyperdiploid (HeH) cases with a trisomy 14 can harbor three rearrangements, a pattern that otherwise may be misinterpreted to be oligoclonal. Oligoclonal IGH rearrangements, on the other hand, may be instable at relapse and should therefore not be used for minimal residual disease analysis. We thus investigated the association between IGH allele copy numbers and the IGH rearrangement patterns in 90 HeH BCP ALL with either two (13%) or three copies (87%) of chromosome 14. HeH cases (44%) had an oligoclonal IGH rearrangement pattern, but true oligoclonality—after correction for the respective copy number of IGH alleles—was only 16%. Monoclonal and oligoclonal HeH cases had predominantly VH to preexisting DJH recombinations, a finding that contrasts with oligoclonal cases of other major genetic BCP ALL subgroups in which VH replacements prevail. We conclude that for the precise assessment and correct interpretation of clonality patterns in BCP ALL, the IGH allele copy number has to be taken into consideration.Leukemia (2009) 23, 870–876; doi:10.1038/leu.2008.390; published online 15 January 2009 [ABSTRACT FROM AUTHOR]

Published

2009

32. TACI mutations and disease susceptibility in patients with common variable immunodeficiency.

Author

Poodt, A. E. J., Driessen, G. J. A., de Klein, A., van Dongen, J. J. M., van der Burg, M., and de Vries, E.

Subjects

IMMUNODEFICIENCY, GENETIC mutation, IMMUNOGLOBULIN A, INFECTION, DISEASE susceptibility, PNEUMOCOCCAL vaccines

Abstract

The most prevalent primary immunodeficiency is common variable immunodeficiency (CVID). Mutations have been described in four genes, ICOS, CD19, BAFF-R and TNFRSF13B (encoding TACI), together associated with 10–15% of CVID cases. We investigated a family with CVID and identified the heterozygous C104R TNFRSF13B mutation in two of the three index-children with CVID, a mother with selective immunoglobulin A deficiency, a mother with recurrent infections and a healthy grandfather. Remarkably, we did not find the TNFRSF13B mutation in the third index-child with CVID, despite his hypogammaglobulinaemia and decreased response to unconjugated pneumococcal vaccine. This family illustrates that TNFRSF13B mutations induce disease susceptibility rather than cause disease directly. Apparently, other genetic or environmental factors, still to be identified, contributed to the development of CVID in this family. Consequently, TNFRSF13B mutations must be interpreted with caution in the clinical setting. [ABSTRACT FROM AUTHOR]

Published

2009

33. Sola dosis facit venenum. Leukemia in gene therapy trials: a question of vectors, inserts and dosage?

Author

Staal, F. J. T., Pike-Overzet, K., Ng, Y. Y., and van Dongen, J. J. M.

Subjects

HTLV, LYMPHOBLASTIC leukemia, GENETIC mutation, RETROVIRUS genetics, TERATOGENESIS

Abstract

In clinical gene therapy trials for X-linked severe combined immunodeficiency, the development of leukemia has come up as a severe adverse effect. In all five cases, T-cell acute lymphoblastic leukemia (T-ALL) occurred as a direct consequence of insertional mutagenesis by the retrovirus used to deliver the therapeutic gene. Here, we review the mechanisms of insertional mutagenesis, the function of the Il2RG gene and the future developments in the field. New lentiviral and gamma retroviral vectors can significantly improve the safety profile of the tools used but still carry the risk of insertional mutagenesis, as shown in this issue of Leukemia. Finally, the unfortunate side effects of gene therapy have given more insight into the development of human T-ALL. [ABSTRACT FROM AUTHOR]

Published

2008

34. Minimal residual disease-directed risk stratification using real-time quantitative PCR analysis of immunoglobulin and T-cell receptor gene rearrangements in the international multicenter trial AIEOP-BFM ALL 2000 for childhood acute lymphoblastic leukemia.

Author

Flohr, T., Schrauder, A., Cazzaniga, G., Panzer-Grümayer, R., van der Velden, V., Fischer, S., Stanulla, M., Basso, G., Niggli, F. K., Schäfer, B. W., Sutton, R., Koehler, R., Zimmermann, M., Valsecchi, M. G., Gadner, H., Masera, G., Schrappe, M., van Dongen, J. J. M., Biondi, A., and Bartram, C. R.

Subjects

POLYMERASE chain reaction, IMMUNOGLOBULINS, T cell receptors, REARRANGEMENTS (Chemistry), LYMPHOBLASTIC leukemia, DISEASE relapse

Abstract

Detection of minimal residual disease (MRD) is the most sensitive method to evaluate treatment response and one of the strongest predictors of outcome in childhood acute lymphoblastic leukemia (ALL). The 10-year update on the I-BFM-SG MRD study 91 demonstrates stable results (event-free survival), that is, standard risk group (MRD-SR) 93%, intermediate risk group (MRD-IR) 74%, and high risk group (MRD-HR) 16%. In multicenter trial AIEOP-BFM ALL 2000, patients were stratified by MRD detection using quantitative PCR after induction (TP1) and consolidation treatment (TP2). From 1 July 2000 to 31 October 2004, PCR target identification was performed in 3341 patients: 2365 (71%) patients had two or more sensitive targets (10−4), 671 (20%) patients revealed only one sensitive target, 217 (6%) patients had targets with lower sensitivity, and 88 (3%) patients had no targets. MRD-based risk group assignment was feasible in 2594 (78%) patients: 40% were classified as MRD-SR (two sensitive targets, MRD negativity at both time points), 8% as MRD-HR (MRD 10−3 at TP2), and 52% as MRD-IR. The remaining 823 patients were stratified according to clinical risk features: HR (n=108) and IR (n=715). In conclusion, MRD-PCR-based stratification using stringent criteria is feasible in almost 80% of patients in an international multicenter trial.Leukemia (2008) 22, 771–782; doi:10.1038/leu.2008.5; published online 31 January 2008 [ABSTRACT FROM AUTHOR]

Published

2008

35. Non-specific amplification of patient-specific Ig/TCR gene rearrangements depends on the time point during therapy: implications for minimal residual disease monitoring.

Author

van der Velden, V. H. J., Wijkhuijs, J. M., and van Dongen, J. J. M.

Subjects

LETTERS to the editor, GENE amplification

Abstract

A letter to the editor is presented regarding the implications of time dependence in immunoglobulin and T-cell receptor amplification, on the monitoring of residual diseases.

Published

2008

36. Childhood secondary ALL after ALL treatment.

Author

Zuna, J, Cavé, H, Eckert, C, Szczepanski, T, Meyer, C, Mejstrikova, E, Fronkova, E, Muzikova, K, Clappier, E, Mendelova, D, Boutard, P, Schrauder, A, Sterba, J, Marschalek, R, van Dongen, J J M, Hrusak, O, Stary, J, and Trka, J

Subjects

LYMPHOBLASTIC leukemia in children, CANCER relapse, LEUKEMIA in children, T-cell receptor genes, JUVENILE diseases, MEDICAL research, LEUKEMIA treatment

Abstract

Data on secondary acute lymphoblastic leukaemia (sALL) following ALL treatment are very rare. However, the incidence might be underestimated as sALLs without a significant lineage shift might automatically be diagnosed as relapses. Examination of immunoglobulin and T-cell receptor gene rearrangements brought a new tool that can help in discrimination between relapse and sALL. We focused on the recurrences of childhood ALL to discover the real frequency of the sALL after ALL treatment. We compared clonal markers in matched presentation and recurrence samples of 366 patients treated according to the Berlin–Frankfurt–Munster (BFM)-based protocols. We found two cases of sALL and another three, where the recurrence is suspicious of being sALL rather than relapse. Our proposal for the ‘secondary ALL after ALL’ diagnostic criteria is as follows: (A) No clonal relationship between diagnosis and recurrence; (B) significant immunophenotypic shift – significant cytogenetic shift – gain/loss of a fusion gene. For the sALL (A) plus at least one (B) criterion should be fulfilled. With these criteria, the estimated frequency of the sALL after ALL is according to our data 0.5–1.5% of ALL recurrences on BFM-based protocols. Finally, we propose a treatment strategy for the patients with secondary disease.Leukemia (2007) 21, 1431–1435; doi:10.1038/sj.leu.2404718; published online 26 April 2007 [ABSTRACT FROM AUTHOR]

Published

2007

37. Ectopic retroviral expression of LMO2, but not IL2Rγ, blocks human T-cell development from CD34+ cells: implications for leukemogenesis in gene therapy.

Author

Pike-Overzet, K., de Ridder, D., Weerkamp, F., Baert, M. R. M., Verstegen, M. M. A., Brugman, M. H., Howe, S. J., Reinders, M. J. T., Thrasher, A. J., Wagemaker, G., van Dongen, J. J. M., and Staal, F. J. T.

Subjects

SEVERE combined immunodeficiency, GENE therapy, INTERLEUKIN-2, T cells, ONCOGENES

Abstract

The occurrence of leukemia in a gene therapy trial for SCID-X1 has highlighted insertional mutagenesis as an adverse effect. Although retroviral integration near the T-cell acute lymphoblastic leukemia (T-ALL) oncogene LIM-only protein 2 (LMO2) appears to be a common event, it is unclear why LMO2 was preferentially targeted. We show that of classical T-ALL oncogenes, LMO2 is most highly transcribed in CD34+ progenitor cells. Upon stimulation with growth factors typically used in gene therapy protocols transcription of LMO2, LYL1, TAL1 and TAN1 is most prominent. Therefore, these oncogenes may be susceptible to viral integration. The interleukin-2 receptor gamma chain (IL2Rγ), which is mutated in SCID-X1, has been proposed as a cooperating oncogene to LMO2. However, we found that overexpressing IL2Rγ had no effect on T-cell development. In contrast, retroviral overexpression of LMO2 in CD34+ cells caused severe abnormalities in T-cell development, but B-cell and myeloid development remained unaffected. Our data help explain why LMO2 was preferentially targeted over many of the other known T-ALL oncogenes. Furthermore, during T-cell development retrovirus-mediated expression of IL2Rγ may not be directly oncogenic. Instead, restoration of normal IL7-receptor signaling may allow progression of T-cell development to stages where ectopic LMO2 expression causes aberrant thymocyte growth.Leukemia (2007) 21, 754–763. doi:10.1038/sj.leu.2404563; published online 1 February 2007 [ABSTRACT FROM AUTHOR]

Published

2007

38. Optimization of PCR-based minimal residual disease diagnostics for childhood acute lymphoblastic leukemia in a multi-center setting.

Author

van der Velden, V. H. J., Panzer-Grümayer, E. R., Cazzaniga, G., Flohr, T., Sutton, R., Schrauder, A., Basso, G., Schrappe, M., Wijkhuijs, J. M., Konrad, M., Bartram, C. R., Masera, G., Biondi, A., and van Dongen, J. J. M.

Subjects

LYMPHOBLASTIC leukemia in children, DIAGNOSTIC use of polymerase chain reaction, IMMUNOGLOBULINS, T-cell receptor genes, QUALITY control

Abstract

Minimal residual disease (MRD) diagnostics is used for treatment stratification in childhood acute lymphoblastic leukemia. We aimed to identify and solve potential problems in multicenter MRD studies to achieve and maintain consistent results between the AIEOP/BFM ALL-2000 MRD laboratories. As the dot-blot hybridization method was replaced by the real-time quantitative polymerase chain reaction (RQ-PCR) method during the treatment protocol, special attention was given to the comparison of MRD data obtained by both methods and to the reproducibility of RQ-PCR data. Evaluation of all key steps in molecular MRD diagnostics identified several pitfalls that resulted in discordant MRD results. In particular, guidelines for RQ-PCR data interpretation appeared to be crucial for obtaining concordant MRD results. The experimental variation of the RQ-PCR was generally less than three-fold, but logically became larger at low MRD levels below the reproducible sensitivity of the assay (<10−4). Finally, MRD data obtained by dot-blot hybridization were comparable to those obtained by RQ-PCR analysis (r2=0.74). In conclusion, MRD diagnostics using RQ-PCR analysis of immunoglobulin/T-cell receptor gene rearrangements is feasible in multicenter studies but requires standardization; particularly strict guidelines for interpretation of RQ-PCR data are required. We further recommend regular quality control for laboratories performing MRD diagnostics in international treatment protocols.Leukemia (2007) 21, 706–713. doi:10.1038/sj.leu.2404535; published online 8 February 2007 [ABSTRACT FROM AUTHOR]

Published

2007

39. Acute lymphoblastic leukemia with t(4;11) in children 1 year and older: The ‘big sister’ of the infant disease?

Author

Mann, G., Cazzaniga, G., van der Velden, V. H. J., Flohr, T., Csinady, E., Paganin, M., Schrauder, A., Dohnal, A. M., Schrappe, M., Biondi, A., Gadner, H., van Dongen, J. J. M., and Panzer-Grümayer, E. R.

Subjects

LYMPHOBLASTIC leukemia in children, IMMUNOGLOBULINS, IMMUNOPHENOTYPING, T-cell receptor genes, B cells, GENE fusion, INFANT diseases

Abstract

The t(4;11)-positive acute lymphoblastic leukemia (ALL) is a rare disease in children above the age of 1 year. We studied the clinical and biological characteristics in 32 consecutively diagnosed childhood cases (median age 10.0 years, range 1.0–17.1 years). Immunophenotyping revealed a pro-B and a pre-B stage in 24 and eight cases, respectively. IGH genes were rearranged in 84% of leukemias with a predominance of incomplete DJH joints. Whereas IGK-Kde and TCRD rearrangements were rare, TCRG rearrangements were present in 50% of cases and involved mainly Vγ11 or Vγ9 together with a Jγ1.3./2.3 gene segment, an unusual combination among t(4;11)-negative B-cell precursor ALL. Oligoclonality was found in about 30% as assessed by heterogeneous IGH and TCRG rearrangements. Our data are in line with transformation of a precursor cell at an early stage of B-cell development but retaining the potential to differentiate to the pre-B cell stage in vivo. Although a distinct difference between infant and older childhood cases with t(4;11) became evident, no age-related biological features were found within the childhood age group. In contrast to infants with t(4;11)-positive ALL, childhood cases had a relatively low cumulative incidence of relapse of 25% at 3.5 years with BFM-based high-risk protocols.Leukemia (2007) 21, 642–646. doi:10.1038/sj.leu.2404577; published online 8 February 2007 [ABSTRACT FROM AUTHOR]

Published

2007

40. Immunobiological diversity in infant acute lymphoblastic leukemia is related to the occurrence and type of MLL gene rearrangement.

Author

Jansen, M. W. J. C., Corral, L., van der Velden, V. H. J., Panzer-Grümayer, R., Schrappe, M., Schrauder, A., Marschalek, R., Meyer, C., den Boer, M. L., Hop, W. J. C., Valsecchi, M. G., Basso, G., Biondi, A., Pieters, R., van Dongen, J. J. M., and Panzer-Grümayer, R

Subjects

LYMPHOBLASTIC leukemia in children, IMMUNOGLOBULINS, IMMUNOPHENOTYPING, T-cell receptor genes, ANTIBODY diversity

Abstract

The aim of this study was to identify immunobiological subgroups in 133 infant acute lymphoblastic leukemia (ALL) cases as assessed by their immunophenotype, immunoglobulin (Ig) and T-cell receptor (TCR) gene rearrangement pattern, and the presence of mixed lineage leukemia (MLL) rearrangements. About 70% of cases showed the pro-B-ALL immunophenotype, whereas the remaining cases were common ALL and pre-B-ALL. MLL translocations were found in 79% of infants, involving MLL-AF4 (41%), MLL-ENL (18%), MLL-AF9 (11%) or another MLL partner gene (10%). Detailed analysis of Ig/TCR rearrangement patterns revealed IGH, IGK and IGL rearrangements in 91, 21 and 13% of infants, respectively. Cross-lineage TCRD, TCRG and TCRB rearrangements were found in 46, 17 and 10% of cases, respectively. As compared to childhood precursor-B-ALL, Ig/TCR rearrangements in infant ALL were less frequent and more oligoclonal. MLL-AF4 and MLL-ENL-positive infants demonstrated immature rearrangements, whereas in MLL-AF9-positive leukemias more mature rearrangements predominated. The immature Ig/TCR pattern in infant ALL correlated with young age at diagnosis, CD10 negativity and predominantly with the presence and the type of MLL translocation. The high frequency of immature and oligoclonal Ig/TCR rearrangements is probably caused by early (prenatal) oncogenic transformation in immature B-lineage progenitor cells with germline Ig/TCR genes combined with a short latency period. [ABSTRACT FROM AUTHOR]

Published

2007

41. Analysis of minimal residual disease by Ig/TCR gene rearrangements: guidelines for interpretation of real-time quantitative PCR data.

Author

van der Velden, V. H. J., Cazzaniga, G., Schrauder, A., Hancock, J., Bader, P., Panzer-Grumayer, E. R., Flohr, T., Sutton, R., Cave, H., Madsen, H. O., Cayuela, J. M., Trka, J., Eckert, C., Foroni, L., zur Stadt, U., Beldjord, K., Raff, T., van der Schoot, C. E., and van Dongen, J. J. M.

Subjects

LYMPHOBLASTIC leukemia treatment, DIAGNOSTIC use of polymerase chain reaction, IMMUNOGLOBULINS, T-cell receptor genes, QUALITY control, GUIDELINES, DRUGS

Abstract

Most modern treatment protocols for acute lymphoblastic leukaemia (ALL) include the analysis of minimal residual disease (MRD). To ensure comparable MRD results between different MRD-polymerase chain reaction (PCR) laboratories, standardization and quality control are essential. The European Study Group on MRD detection in ALL (ESG-MRD-ALL), consisting of 30 MRD-PCR laboratories worldwide, has developed guidelines for the interpretation of real-time quantitative PCR-based MRD data. The application of these guidelines ensures identical interpretation of MRD data between different laboratories of the same MRD-based clinical protocol. Furthermore, the ESG-MRD-ALL guidelines will facilitate the comparison of MRD data obtained in different treatment protocols, including those with new drugs.Leukemia (2007) 21, 604–611. doi:10.1038/sj.leu.2404586; published online 8 February 2007 [ABSTRACT FROM AUTHOR]

Published

2007

42. Human T-cell lines with well-defined T-cell receptor gene rearrangements as controls for the BIOMED-2 multiplex polymerase chain reaction tubes.

Author

Sandberg, Y., Verhaaf, B., van Gastel-Mol, E. J., Wolvers-Tettero, I. L. M., de Vos, J., MacLeod, R. A. F., Noordzij, J. G., Dik, W. A., van Dongen, J. J. M., and Langerak, A. W.

Subjects

POLYMERASE chain reaction, T-cell receptor genes, IMMUNOGLOBULIN genes, CELL lines, T cells, LEUKEMIA

Abstract

The BIOMED-2 multiplex polymerase chain reaction (PCR) tubes for analysis of immunoglobulin and T-cell receptor (TCR) gene rearrangements have recently been introduced as a reliable and easy tool for clonality diagnostics in suspected lymphoproliferations. Quality and performance assessment of PCR-based clonality diagnostics is generally performed using human leukemia/lymphoma cell lines as controls. We evaluated the utility of 30 well-defined human T-cell lines for quality performance testing of the BIOMED-2 PCR primers and protocols. The PCR analyses of the TCR loci were backed up by Southern blot analysis. The clonal TCRB, TCRG and TCRD gene rearrangements were analyzed for gene segment usage and for the size and composition of their junctional regions. In 29 out of 30 cell lines, unique clonal TCR gene rearrangements could be easily detected. Besides their usefulness in molecular clonality diagnostics, these cell lines can now be authenticated based on their TCR gene rearrangement profile. This enables their correct use in molecular clonality diagnostics and in other cancer research studies.Leukemia (2007) 21, 230–237. doi:10.1038/sj.leu.2404486; published online 14 December 2006 [ABSTRACT FROM AUTHOR]

Published

2007

43. Polymerase chain reaction-based clonality testing in tissue samples with reactive lymphoproliferations: usefulness and pitfalls. A report of the BIOMED-2 Concerted Action BMH4-CT98-3936.

Author

Langerak, A. W., Molina, T. J., Lavender, F. L., Pearson, D., Flohr, T., Sambade, C., Schuuring, E., Al Saati, T., van Dongen, J. J .M., and van Krieken, J. H. J. M.

Subjects

LYMPHOPROLIFERATIVE disorders, DIAGNOSTIC use of polymerase chain reaction, LYMPHOMAS, T cell receptors, IMMUNOHISTOCHEMISTRY, DIAGNOSIS

Abstract

Lymphoproliferations are generally diagnosed via histomorphology and immunohistochemistry. Although mostly conclusive, occasionally the differential diagnosis between reactive lesions and malignant lymphomas is difficult. In such cases molecular clonality studies of immunoglobulin (Ig)/T-cell receptor (TCR) rearrangements can be useful. Here we address the issue of clonality assessment in 106 histologically defined reactive lesions, using the standardized BIOMED-2 Ig/TCR multiplex polymerase chain reaction (PCR) heteroduplex and GeneScan assays. Samples were reviewed nationally, except 10% random cases and cases with clonal results selected for additional international panel review. In total 75% (79/106) only showed polyclonal Ig/TCR targets (type I), whereas another 15% (16/106) represent probably polyclonal cases, with weak Ig/TCR (oligo)clonality in an otherwise polyclonal background (type II). Interestingly, in 10% (11/106) clear monoclonal Ig/TCR products were observed (types III/IV), which prompted further pathological review. Clonal cases included two missed lymphomas in national review and nine cases that could be explained as diagnostically difficult cases or probable lymphomas upon additional review. Our data show that the BIOMED-2 Ig/TCR multiplex PCR assays are very helpful in confirming the polyclonal character in the vast majority of reactive lesions. However, clonality detection in a minority should lead to detailed pathological review, including close interaction between pathologist and molecular biologist.Leukemia (2007) 21, 222–229. doi:10.1038/sj.leu.2404482; published online 14 December 2006 [ABSTRACT FROM AUTHOR]

Published

2007

44. Identification of Notch target genes in uncommitted T-cell progenitors: No direct induction of a T-cell specific gene program.

Author

Weerkamp, F., Luis, T. C., Naber, B. A. E., Koster, E. E. L., Jeannotte, L., van Dongen, J. J. M., and Staal, F. J. T.

Subjects

NOTCH genes, T-cell receptor genes, LYMPHOBLASTIC leukemia, GENE expression, CANCER genetics, HEMATOPOIETIC stem cells

Abstract

Deregulated Notch signaling occurs in the majority of human T-ALL. During normal lymphoid development, activation of the Notch signaling pathway poses a T-cell fate on hematopoietic progenitors. However, the transcriptional targets of the Notch pathway are largely unknown. We sought to identify Notch target genes by inducing Notch signaling in human hematopoietic progenitors using two different methods: an intracellular signal through transfection of activated Notch and a Notch-receptor dependent signal by interaction with its ligand Delta1. Gene expression profiles were generated and evaluated with respect to expression profiles of immature thymic subpopulations. We confirmed HES1, NOTCH1 and NRARP as Notch target genes, but other reported Notch targets, including the genes for Deltex1, pre-T-cell receptor alpha and E2A, were not found to be differentially expressed. Remarkably, no induction of T-cell receptor gene rearrangements or transcription of known T-cell specific genes was found after activation of the Notch pathway. A number of novel Notch target genes, including the transcription factor TCFL5 and the HOXA cluster, were identified and functionally tested. Apparently, Notch signaling is essential to open the T-cell pathway, but does not initiate the T-cell program itself. [ABSTRACT FROM AUTHOR]

Published

2006

45. Consensus guidelines for microarray gene expression analyses in leukemia from three European leukemia networks.

Author

Staal, F. J. T., Cario, G., Cazzaniga, G., Haferlach, T., Heuser, M., Hofmann, W.-K., Mills, K., Schrappe, M., Stanulla, M., Wingen, L. U., van Dongen, J. J. M., and Schlegelberger, B.

Subjects

GENE expression, LEUKEMIA, DNA, HEMATOLOGY, LYMPHOMAS, TUMORS

Abstract

A plethora of studies have documented that gene expression profiling using DNA microarrays for various types of hematological malignancies provides novel information, which may have diagnostic and prognostic implications. However, to successfully use microarrays for this purpose, the quality and reproducibility of the whole procedure need to be guaranteed. Critical steps of the method are handling, processing and storage of the leukemic sample, purification of tumor cells (or lack thereof), RNA extraction methods, quality control of RNA, labeling techniques, hybridization, washing, scanning, spot filtering, normalization and initial interpretation, and finally the biostatistical analysis. These items have been extensively discussed and evaluated in different multi-center quality rounds within the three networks, that is, I-BFM-SG, the German Competence Network ‘Acute and Chronic Leukemias’ and the European LeukemiaNet. Based on the exchange of knowledge and experience between the three networks over the last few years, we have formulated guidelines for performing microarray experiments in leukemia. We confine ourselves to leukemias, but many of these requirements also apply to lymphomas or other clinical samples, including solid tumors.Leukemia (2006) 20, 1385–1392. doi:10.1038/sj.leu.2404274; published online 8 June 2006 [ABSTRACT FROM AUTHOR]

Published

2006

46. Notch and Wnt signaling in T-lymphocyte development and acute lymphoblastic leukemia.

Author

Weerkamp, F, van Dongen, J J M, and Staal, F J T

Subjects

HTLV, T cells, LYMPHOCYTES, NOTCH genes, LYMPHOBLASTIC leukemia

Abstract

Many acute lymphoblastic leukemias can be considered as malignant counterparts of cells in the various stages of normal lymphoid development in bone marrow and thymus. T-cell development in the thymus is an ordered and tightly controlled process. Two evolutionary conserved signaling pathways, which were first discovered in Drosophila, control the earliest steps of T-cell development. These are the Notch and Wnt-signaling routes, which both are deregulated in several types of leukemias. In this review we discuss both pathways, with respect to their signaling mechanisms, functions during T-cell development and their roles in development of leukemias, especially T-cell acute lymphoblastic leukemia.Leukemia (2006) 20, 1197–1205. doi:10.1038/sj.leu.2404255; published online 11 May 2006 [ABSTRACT FROM AUTHOR]

Published

2006

47. The MLL recombinome of acute leukemias.

Author

Meyer, C., Schneider, B., Jakob, S., Strehl, S., Attarbaschi, A., Schnittger, S., Schoch, C., Jansen, M. W. J. C., van Dongen, J. J. M., den Boer, M. L., Pieters, R., Ennas, M.-G., Angelucci, E., Koehl, U., Greil, J., Griesinger, F., zur Stadt, U., Eckert, C., Szczepański, T., and Niggli, F. K.

Subjects

ACUTE leukemia, LEUKEMIA in children, MYELOID leukemia, CHROMOSOMES, PEDIATRICS, PROTEIN metabolism, CHROMOSOME abnormalities, COMPARATIVE studies, DNA, GENE mapping, LEUKEMIA, RESEARCH methodology, MEDICAL cooperation, METHYLATION, PROTEINS, RESEARCH, TRANSFERASES, EVALUATION research, ACUTE diseases

Abstract

Chromosomal rearrangements of the human MLL gene are a hallmark for aggressive (high-risk) pediatric, adult and therapy-associated acute leukemias. These patients need to be identified in order to subject these patients to appropriate therapy regimen. A recently developed long-distance inverse PCR method was applied to genomic DNA isolated from individual acute leukemia patients in order to identify chromosomal rearrangements of the human MLL gene. We present data of the molecular characterization of 414 samples obtained from 272 pediatric and 142 adult leukemia patients. The precise localization of genomic breakpoints within the MLL gene and the involved translocation partner genes (TPGs) was determined and several new TPGs were identified. The combined data of our study and published data revealed a total of 87 different MLL rearrangements of which 51 TPGs are now characterized at the molecular level. Interestingly, the four most frequently found TPGs (AF4, AF9, ENL and AF10) encode nuclear proteins that are part of a protein network involved in histone H3K79 methylation. Thus, translocations of the MLL gene, by itself coding for a histone H3K4 methyltransferase, are presumably not randomly chosen, rather functionally selected. [ABSTRACT FROM AUTHOR]

Published

2006

48. TCRγδ+ large granular lymphocyte leukemias reflect the spectrum of normal antigen-selected TCRγδ+ T-cells.

Author

Sandberg, Y., Almeida, J., Gonzalez, M., Lima, M., Bárcena, P., Szczepañski, T., van Gastel-Mol, E. J., Wind, H., Balanzategui, A., van Dongen, J. J. M., Miguel, J. F. San, Orfao, A., and Langerak, A. W.

Subjects

T cells, LYMPHOCYTES, ANTIGENS, LYMPHOCYTIC leukemia, BLOOD diseases, CANCER patients, NEUTROPENIA, ANEMIA

Abstract

T-cell large granular lymphocytes (LGL) proliferations range from reactive expansions of activated T cells to T-cell leukemias and show variable clinical presentation and disease course. The vast majority of T-LGL proliferations express TCRαβ. Much less is known about the characteristics and pathogenesis of TCRγδ+ cases. We evaluated 44 patients with clonal TCRγδ+ T-LGL proliferations with respect to clinical data, immunophenotype and TCR gene rearrangement pattern. TCRγδ+ T-LGL leukemia patients had similar clinical presentations as TCRαβ+ T-LGL leukemia patients. Their course was indolent and 61% of patients were symptomatic. The most common clinical manifestations were chronic cytopenias – neutropenia (48%), anemia (23%), thrombocytopenia (9%), pancytopenia (2%) – and to a lesser extent splenomegaly (18%). Also multiple associated autoimmune (34%) and hematological (14%) disorders were found. Leukemic LGLs were predominantly positive for CD2, CD5, CD7, CD8, and CD57, whereas variable expression was seen for CD16, CD56, CD11b, and CD11c. The Vγ9/Vδ2 immunophenotype was found in 48% of cases and 43% of cases was positive for Vδ1, reflecting the TCR-spectrum of normal TCRγδ+ T-cells in adult PB. Identification of the well-defined post-thymic Vδ2-Jδ1 selection determinant in all evaluable Vγ9+/Vδ2+ patients, is suggestive of common (super)antigen involvement in the pathogenesis of these TCRγδ+ T-LGL leukemia patients.Leukemia (2006) 20, 505–513. doi:10.1038/sj.leu.2404112; published online 26 January 2006 [ABSTRACT FROM AUTHOR]

Published

2006

49. CALM-AF10+ T-ALL expression profiles are characterized by overexpression of HOXA and BMI1 oncogenes.

Author

Dik, W. A., Brahim, W., Braun, C., Asnafi, V., Dastugue, N., Bernard, O. A., van Dongen, J. J. M., Langerak, A. W., Macintyre, E. A., and Delabesse, E.

Subjects

ACUTE myeloid leukemia, PROTEIN microarrays, POLYMERASE chain reaction, REVERSE transcriptase, TUMOR suppressor genes, LEUKEMIA etiology

Abstract

The t(10;11)(p13;q14-21) is found in T-ALL and acute myeloid leukemia and fuses CALM (Clathrin-Assembly protein-like Lymphoid-Myeloid leukaemia gene) to AF10. In order to gain insight into the transcriptional consequences of this fusion, microarray-based comparison of CALM-AF10+ vs CALM-AF10- T-ALL was performed. This analysis showed upregulation of HOXA5, HOXA9, HOXA10 and BMI1 in the CALM-AF10+ cases. Microarray results were validated by quantitative RT-PCR on an independent group of T-ALL and compared to mixed lineage leukemia-translocated acute leukemias (MLL-t AL). The overexpression of HOXA genes was associated with overexpression of its cofactor MEIS1 in CALM-AF10+ T-ALL, reaching levels of expression similar to those observed in MLL-t AL. Consequently, CALM-AF10+ T-ALL and MLL-t AL share a specific HOXA overexpression, indicating they activate common oncogenic pathways. In addition, BMI1, located close to AF10 breakpoint, was overexpressed only in CALM-AF10+ T-ALL and not in MLL-t AL. BMI1 controls cellular proliferation through suppression of the tumor suppressors encoded by the CDKN2A locus. This locus, often deleted in T-ALL, was conserved in CALM-AF10+ T-ALL. This suggests that decreased CDKN2A activity, as a result of BMI1 overexpression, contributes to leukemogenesis in CALM-AF10+ T-ALL. We propose to define a HOXA+ leukemia group composed of at least MLL-t, CALM-AF10 and HOXA-t AL, which may benefit from adapted management. [ABSTRACT FROM AUTHOR]

Published

2005

50. Split-signal FISH for detection of chromosome aberrations.

Author

van Dongen, J. J. M, van der Burg, M, and Langerak, A. W

Subjects

CHROMOSOMES, HEMATOPOIETIC system, ONCOGENES, LEUKEMIA, THERAPEUTICS, KARYOTYPES

Abstract

Chromosome aberrations are frequently observed in hematopoietic malignancies. These aberrations can deregulate expression of an oncogene, resulting in aberrant expression or overexpression, or they can form leukemia-specific chimeric fusion proteins. Detection of chromosome aberrations is an important tool for classification of the malignancy and for the definition of risk groups, which need different treatment protocols. We developed rapid and sensitive split-signal fluorescent in situ hybridization (FISH) assays for frequently occuring chromosome aberrations. The split-signal FISH approach uses two differentially labeled probes, located in one gene at opposite sites of the breakpoint region. In normal karyotypes, two co-localized green/red signals are visible, but a translocation results in a split of one of the co-localized signals. Split-signal FISH has three main advantages over the classical fusion-signal FISH approach, which uses of two labeled probes located in two genes. First, the detection of a chromosome aberration is independent of the involved partner gene. Second, split-signal FISH allows the identification of the partner gene or chromosome region if metaphase spreads are present, and finally it reduces false-positivity. [ABSTRACT FROM AUTHOR]

Published

2005