Your search keyword '"pre-B cells"' showing total 83 results

1. DNA damage–induced p53 downregulates expression of RAG1 through a negative feedback loop involving miR-34a and FOXP1

Author

Ochodnicka-Mackovicova, Katarina, van Keimpema, Martine, Spaargaren, Marcel, van Noesel, Carel J.M., and Guikema, Jeroen E.J.

Published

2024

2. Dysregulation of B lymphocyte development in the SKG mouse model of rheumatoid arthritis.

Author

Kim, Joo Eun, Tung, Lin Tze, Jiang, Roselyn R., Yousefi, Mitra, Liang, Yue, Malo, Danielle, Vidal, Silvia M., and Nijnik, Anastasia

Subjects

*B cells, *RHEUMATOID arthritis, *COLONY-forming units assay, *BONE marrow cells, *LABORATORY mice, *AGAMMAGLOBULINEMIA, *PURE red cell aplasia

Abstract

Rheumatoid arthritis is a chronic and systemic inflammatory disease that affects approximately 1% of the world's population and is characterised by joint inflammation, the destruction of articular cartilage and bone, and many potentially life‐threatening extraarticular manifestations. B lymphocytes play a central role in the pathology of rheumatoid arthritis as the precursors of autoantibody secreting plasma cells, as highly potent antigen‐presenting cells, and as a source of various inflammatory cytokines, however, the effects of rheumatoid arthritis on B lymphocyte development remain poorly understood. Here, we analyse B lymphocyte development in murine models of rheumatoid arthritis, quantifying all the subsets of B cell precursors in the bone marrow and splenic B cells using flow cytometry. We demonstrate a severe reduction in pre‐B cells and immature B cells in the bone marrow of mice with active disease, despite no major effects on the mature naïve B cell numbers. The loss of B cell precursors in the bone marrow of the affected mice was associated with a highly significant reduction in the proportion of Ki67+ cells, indicating impaired cell proliferation, while the viability of the B cell precursors was not significantly affected. We also observed some mobilisation of the B cell precursor cells into the mouse spleen, demonstrated with flow cytometry and pre‐B colony forming units assays. In summary, the current work demonstrates a severe dysregulation in B lymphocyte development in murine rheumatoid arthritis, with possible implications for B cell repertoire formation, tolerance induction, and disease mechanisms. [ABSTRACT FROM AUTHOR]

Published

2023

3. High Salt-Induced Hyperosmolality Reduces in Vitro Survival and Proliferation of Pre-B Cells.

Author

Yabas, Mehmet

Subjects

INTERLEUKINS, IN vitro studies, FLOW cytometry, B cells, CELL culture, ANIMAL experimentation, APOPTOSIS, CELL survival, CELLULAR signal transduction, CELL proliferation, OSMOLAR concentration, TRANSCRIPTION factors, BONE marrow, DIETARY sodium, MICE

Abstract

Aim: B cells of the adaptive immunity are critical for protection against the vast majority of pathogens through the production of specific antibodies. A number of signaling pathways and transcription factors control B cell development. Environmental factors, including diet, are also important in determining how B cell develop and function. Here, the effects of hyperosmolality induced by elevated salt on the survival, IL-7-induced proliferation and differentiation of pre-B cells were tested in vitro. Material and Methods: The wk3 pre-B cell line generated from SLP65-/- mice was used. Hyperosmolality in the cell culture medium was created by increasing the salt concentration with the addition of 40 mM NaCl. Wk3 pre-B cells were cultured in standard (normal NaCl) and high salt (+40 mM NaCl) medium, followed by flow cytometric analysis. Results: It was found that hyperosmolality caused by high salt reduced survival and induced apoptosis in wk3 pre-B cells. In addition, hyperosmolality inhibited IL-7-induced proliferation of pre-B cells. Conversely, pre-B cells treated with high salt were able to differentiate normally into IgM+ immature B cells when IL-7 was removed. Conclusion: These findings suggest that the hyperosmolar microenvironment induced by high salt may play a key role in B cell development in the bone marrow. [ABSTRACT FROM AUTHOR]

Published

2023

4. ATP11C promotes the differentiation of pre-B cells into immature B cells but does not affect their IL-7-dependent proliferation.

Author

Yabas, Mehmet, Bostanci, Ayten, and Aral, Seda

Abstract

The P4-type ATPases are believed to function as flippases that contribute to the organization of the asymmetric aminophospholipid distribution on the plasma membranes of eukaryotes by their ability to internalize specific phospholipids from the outer leaflet to the inner leaflet. Despite the existence of 14 members of the P4-type ATPases in humans and 15 in mice, their roles in the immune system have not been fully understood. So far, ATP11C was shown to be important for B cells, and mice deficient for ATP11C had a developmental arrest at the pro-B to pre-B cell transition stage of B cell development. Using an ATP11C-deficient pre-B cell line generated through CRISPR/Cas9 engineering, we here tested the role of ATP11C in pre-B cells in vitro and showed that ablation of ATP11C in pre-B cells causes a defect in the flippase activity. We further demonstrated that loss of ATP11C does not impede the proliferation of pre-B cells in response to IL-7. However, pre-B cells lacking ATP11C failed to differentiate into immature B cells upon removal of IL-7. These results suggest that disruption of lipid asymmetry by loss of ATP11C in pre-B cells may control the switch from proliferation to differentiation in pre-B cells. [ABSTRACT FROM AUTHOR]

Published

2023

5. ARID5B regulates fatty acid metabolism and proliferation at the Pre-B cell stage during B cell development.

Author

Chalise, Jaya Prakash, Ehsani, Ali, Lemecha, Mengistu, Yu-Wen Hung, Guoxiang Zhang, Larson, Garrett P., and Itakura, Keiichi

Subjects

B cells, CELL proliferation, FATTY acids, BONE marrow cells, FATTY acid oxidation, PRELEUKEMIA

Abstract

During B cell development in bone marrow, large precursor B cells (large Pre-B cells) proliferate rapidly, exit the cell cycle, and differentiate into non-proliferative (quiescent) small Pre-B cells. Dysregulation of this process may result in the failure to produce functional B cells and pose a risk of leukemic transformation. Here, we report that AT rich interacting domain 5B (ARID5B), a B cell acute lymphoblastic leukemia (B-ALL) risk gene, regulates B cell development at the Pre-B stage. In both mice and humans, we observed a significant upregulation of ARID5B expression that initiates at the Pre-B stage and is maintained throughout later stages of B cell development. In mice, deletion of Arid5b in vivo and ex vivo exhibited a significant reduction in the proportion of immature B cells but an increase in large and small Pre-B cells. Arid5b inhibition ex vivo also led to an increase in proliferation of both Pre-B cell populations. Metabolic studies in mouse and human bone marrow revealed that fatty acid uptake peaked in proliferative B cells then decreased during non-proliferative stages. We showed that Arid5b ablation enhanced fatty acid uptake and oxidation in Pre-B cells. Furthermore, decreased ARID5B expression was observed in tumor cells from B-ALL patients when compared to B cells from non-leukemic individuals. In B-ALL patients, ARID5B expression below the median was associated with decreased survival particularly in subtypes originating from Pre-B cells. Collectively, our data indicated that Arid5b regulates fatty acid metabolism and proliferation of Pre-B cells in mice, and reduced expression of ARID5B in humans is a risk factor for B cell leukemia. [ABSTRACT FROM AUTHOR]

Published

2023

6. ARID5B regulates fatty acid metabolism and proliferation at the Pre-B cell stage during B cell development

Author

Jaya Prakash Chalise, Ali Ehsani, Mengistu Lemecha, Yu-Wen Hung, Guoxiang Zhang, Garrett P. Larson, and Keiichi Itakura

Subjects

ARID5B, B cell development, pre-B cells, fatty acid metabolism, B-ALL, Immunologic diseases. Allergy, RC581-607

Abstract

During B cell development in bone marrow, large precursor B cells (large Pre-B cells) proliferate rapidly, exit the cell cycle, and differentiate into non-proliferative (quiescent) small Pre-B cells. Dysregulation of this process may result in the failure to produce functional B cells and pose a risk of leukemic transformation. Here, we report that AT rich interacting domain 5B (ARID5B), a B cell acute lymphoblastic leukemia (B-ALL) risk gene, regulates B cell development at the Pre-B stage. In both mice and humans, we observed a significant upregulation of ARID5B expression that initiates at the Pre-B stage and is maintained throughout later stages of B cell development. In mice, deletion of Arid5b in vivo and ex vivo exhibited a significant reduction in the proportion of immature B cells but an increase in large and small Pre-B cells. Arid5b inhibition ex vivo also led to an increase in proliferation of both Pre-B cell populations. Metabolic studies in mouse and human bone marrow revealed that fatty acid uptake peaked in proliferative B cells then decreased during non-proliferative stages. We showed that Arid5b ablation enhanced fatty acid uptake and oxidation in Pre-B cells. Furthermore, decreased ARID5B expression was observed in tumor cells from B-ALL patients when compared to B cells from non-leukemic individuals. In B-ALL patients, ARID5B expression below the median was associated with decreased survival particularly in subtypes originating from Pre-B cells. Collectively, our data indicated that Arid5b regulates fatty acid metabolism and proliferation of Pre-B cells in mice, and reduced expression of ARID5B in humans is a risk factor for B cell leukemia.

Published

2023

7. Early B Cell Development

Author

Eibel, Hermann, Emmi, Lorenzo, Series editor, Prisco, Domenico, Series editor, Plebani, Alessandro, editor, and Lougaris, Vassilios, editor

Published

2015

8. Transcriptional Control of Pre-B Cell Development and Leukemia Prevention

Author

Pang, Swee Heng Milon, Carotta, Sebastian, Nutt, Stephen L., Compans, Richard W, Series editor, Cooper, Max D., Series editor, Gleba, Yuri Y., Series editor, Honjo, Tasuku, Series editor, Oldstone, Michael B. A., Series editor, Vogt, Peter K., Series editor, Malissen, Bernard, Series editor, Aktories, Klaus, Series editor, Kawaoka, Yoshihiro, Series editor, Rappuoli, Rino, Series editor, Galan, Jorge E., Series editor, Ahmed, Rafi, Series editor, Ellmeier, Wilfried, editor, and Taniuchi, Ichiro, editor

Published

2014

9. The Role of the Pre-B Cell Receptor in B Cell Development, Repertoire Selection, and Tolerance

Author

Thomas H. Winkler and Inga-Lill Mårtensson

Subjects

surrogate light chain, pre-B cells, B-cell development, allelic exclusion, VpreB, λ-5, Immunologic diseases. Allergy, RC581-607

Abstract

Around four decades ago, it had been observed that there were cell lines as well as cells in the fetal liver that expressed antibody μ heavy (μH) chains in the apparent absence of bona fide light chains. It was thus possible that these cells expressed another molecule(s), that assembled with μH chains. The ensuing studies led to the discovery of the pre-B cell receptor (pre-BCR), which is assembled from Ig μH and surrogate light (SL) chains, together with the signaling molecules Igα and β. It is expressed on a fraction of pro-B (pre-BI) cells and most large pre-B(II) cells, and has been implicated in IgH chain allelic exclusion and down-regulation of the recombination machinery, assessment of the expressed μH chains and shaping the IgH repertoire, transition from the pro-B to pre-B stage, pre-B cell expansion, and cessation.

Published

2018

10. Epigenetic Enhancer Marks and Transcription Factor Binding Influence Vκ Gene Rearrangement in Pre-B Cells and Pro-B Cells

Author

Eden Kleiman, Salvatore Loguercio, and Ann J. Feeney

Subjects

repertoire, enhancer, V(D)J recombination, pro-B cells, pre-B cells, immunoglobulin, Immunologic diseases. Allergy, RC581-607

Abstract

To date there has not been a study directly comparing relative Igκ rearrangement frequencies obtained from genomic DNA (gDNA) and cDNA and since each approach has potential biases, this is an important issue to clarify. Here we used deep sequencing to compare the unbiased gDNA and RNA Igκ repertoire from the same pre-B cell pool. We find that ~20% of Vκ genes have rearrangement frequencies ≥2-fold up or down in RNA vs. DNA libraries, including many members of the Vκ3, Vκ4, and Vκ6 families. Regression analysis indicates Ikaros and E2A binding are associated with strong promoters. Within the pre-B cell repertoire, we observed that individual Vκ genes rearranged at very different frequencies, and also displayed very different Jκ usage. Regression analysis revealed that the greatly unequal Vκ gene rearrangement frequencies are best predicted by epigenetic marks of enhancers. In particular, the levels of newly arising H3K4me1 peaks associated with many Vκ genes in pre-B cells are most predictive of rearrangement levels. Since H3K4me1 is associated with long range chromatin interactions which are created during locus contraction, our data provides mechanistic insight into unequal rearrangement levels. Comparison of Igκ rearrangements occurring in pro-B cells and pre-B cells from the same mice reveal a pro-B cell bias toward usage of Jκ-distal Vκ genes, particularly Vκ10-96 and Vκ1-135. Regression analysis indicates that PU.1 binding is the highest predictor of Vκ gene rearrangement frequency in pro-B cells. Lastly, the repertoires of iEκ−/− pre-B cells reveal that iEκ actively influences Vκ gene usage, particularly Vκ3 family genes, overlapping with a zone of iEκ-regulated germline transcription. These represent new roles for iEκ in addition to its critical function in promoting overall Igκ rearrangement. Together, this study provides insight into many aspects of Igκ repertoire formation.

Published

2018

11. The Role of the Pre-B Cell Receptor in B Cell Development, Repertoire Selection, and Tolerance.

Author

Winkler, Thomas H. and Mårtensson, Inga-Lill

Abstract

Around four decades ago, it had been observed that there were cell lines as well as cells in the fetal liver that expressed antibody μ heavy (μH) chains in the apparent absence of bona fide light chains. It was thus possible that these cells expressed another molecule(s), that assembled with μH chains. The ensuing studies led to the discovery of the pre-B cell receptor (pre-BCR), which is assembled from Ig μH and surrogate light (SL) chains, together with the signaling molecules Igα and β. It is expressed on a fraction of pro-B (pre-BI) cells and most large pre-B(II) cells, and has been implicated in IgH chain allelic exclusion and down-regulation of the recombination machinery, assessment of the expressed μH chains and shaping the IgH repertoire, transition from the pro-B to pre-B stage, pre-B cell expansion, and cessation. [ABSTRACT FROM AUTHOR]

Published

2018

12. Epigenetic Enhancer Marks and Transcription Factor Binding Influence Vκ Gene Rearrangement in Pre-B Cells and Pro-B Cells.

Author

Kleiman, Eden, Loguercio, Salvatore, and Feeney, Ann J.

Subjects

EPIGENETICS, TRANSCRIPTION factors, B cells

Abstract

To date there has not been a study directly comparing relative Igκ rearrangement frequencies obtained from genomic DNA (gDNA) and cDNA and since each approach has potential biases, this is an important issue to clarify. Here we used deep sequencing to compare the unbiased gDNA and RNA Igκ repertoire from the same pre-B cell pool. We find that ~20% of Vκ genes have rearrangement frequencies ≥2-fold up or down in RNA vs. DNA libraries, including many members of the Vκ3, Vκ4, and Vκ6 families. Regression analysis indicates Ikaros and E2A binding are associated with strong promoters. Within the pre-B cell repertoire, we observed that individual Vκ genes rearranged at very different frequencies, and also displayed very different Jκ usage. Regression analysis revealed that the greatly unequal Vκ gene rearrangement frequencies are best predicted by epigenetic marks of enhancers. In particular, the levels of newly arising H3K4me1 peaks associated with many Vκ genes in pre-B cells are most predictive of rearrangement levels. Since H3K4me1 is associated with long range chromatin interactions which are created during locus contraction, our data provides mechanistic insight into unequal rearrangement levels. Comparison of Igκ rearrangements occurring in pro-B cells and pre-B cells from the same mice reveal a pro-B cell bias toward usage of Jκ-distal Vκ genes, particularly Vκ10-96 and Vκ1-135. Regression analysis indicates that PU.1 binding is the highest predictor of Vκ gene rearrangement frequency in pro-B cells. Lastly, the repertoires of iEκ−/− pre-B cells reveal that iEκ actively influences Vκ gene usage, particularly Vκ3 family genes, overlapping with a zone of iEκ-regulated germline transcription. These represent new roles for iEκ in addition to its critical function in promoting overall Igκ rearrangement. Together, this study provides insight into many aspects of Igκ repertoire formation. [ABSTRACT FROM AUTHOR]

Published

2018

13. Deficiency of XLF and PAXX prevents DNA double-strand break repair by non-homologous end joining in lymphocytes.

Author

Hung, Putzer J., Chen, Bo-Ruei, George, Rosmy, Liberman, Caleb, Morales, Abigail J., Colon-Ortiz, Pedro, Tyler, Jessica K., Sleckman, Barry P., and Bredemeyer, Andrea L.

Published

2017

14. Flow cytometry of v-Abl transformed pre-B cells heterogeneous in ectopic expression levels reveals Ras dose–response

Author

Peacock, Ryan W.S., Lawhorn, Ingrid E.B., Ferreira, Joshua P., and Wang, Clifford L.

Subjects

*FLOW cytometry, *B cells, *CELL populations, *GENE expression, *PHOSPHORYLATION, *DOSE-response relationship in biochemistry, *MITOGEN-activated protein kinases

Abstract

Abstract: Flow cytometry is a powerful tool for quantitative biology because it can perform single-cell analysis of large cell populations using multiple parameters. Results are often visualized as a two-dimensional scatter or contour plot. Because these plots can be relatively diffuse, it is not always straightforward to discern a relationship between measured parameters. We have demonstrated that quantitative trends can be fit to the single-cell data generated from a heterogeneous population. We engineered Abelson virus-transformed pre-B cells to express a broad range of oncogenic Ras levels. Instead of individual cultures with individual expression levels, a continuous range of levels was expressed by different cells in one heterogeneous culture. We then stained cells for downstream Erk phosphorylation to monitor MAPK signaling or employed an E2F-responsive genetic reporter to monitor cell-cycle activity. Subsequent analysis by flow cytometry and locally weighted scatterplot smoothing (LOWESS) revealed that increasing Ras oncogene expression led to increasing MAPK signaling. In contrast, E2F activity peaked at an optimal, intermediate level of Ras. To make this analytical method widely available to others, we have provided a software application that performs LOWESS on any two-parameter population data collected by flow cytometry. [Copyright &y& Elsevier]

Published

2012

15. B-cell development in bovine fetuses proceeds via a pre-B like cell in bone marrow and lymph nodes

Author

Ekman, Anna, Pessa-Morikawa, Tiina, Liljavirta, Jenni, Niku, Mikael, and Iivanainen, Antti

Subjects

*CELL growth, *BONE marrow cells, *FETAL cattle, *LYMPH nodes, *IMMUNOHISTOCHEMISTRY, *POLYMERASE chain reaction, *IMMUNOGLOBULINS, *GESTATIONAL age, *GENETIC recombination

Abstract

Abstract: The production of B cells and the primary antibody repertoire in mammalian species other than rodents or man appears to depend on gut-associated lymphoid tissue. Bovine B cells are generated in ileal Peyer''s patch from late gestational to juvenile age. However, little is known about where and when the bona fide B lymphopoiesis takes place. We analyzed bovine fetuses for signs of ongoing B lymphopoiesis using a combination of immunohistochemistry, flow cytometry, real-time quantitative PCR and RNA in situ hybridization. In fetal bone marrow and lymph node, we could demonstrate pre-B like cells positive for intracellular Ig μ but negative for membrane IgM. Strong expression of immunoglobulin lambda-like polypeptide 1 and recombination activating genes was also detected in the same tissues. Similar analyses did not reveal pre-B like cells in the corresponding adult tissues. These results suggest that bovine fetal bone marrow and lymph node support B lymphopoiesis via a pre-B cell like stage before and in parallel to the development of the ileal Peyer''s patch. [Copyright &y& Elsevier]

Published

2010

16. IL-15 inhibits pre-B cell proliferation by selectively expanding Mac-1+B220+ NK cells

Author

Nakajima, Shinsuke, Hida, Shigeaki, and Taki, Shinsuke

Subjects

*KILLER cells, *CELL-mediated cytotoxicity, *IMMUNOCOMPETENT cells, *CELL proliferation

Abstract

Abstract: Natural killer (NK) cells are the cells critical for inhibition of repopulation of allogenic bone marrow cells. However, it is not well known if NK cells affect autologous lymphopoiesis. Here, we observed that NK cells could inhibit pre-B cell proliferation in vitro driven by interleukin (IL)-7 in a manner dependent on IL-15. Interestingly, the great majority of expanding NK cells were Mac-1+B220+, a recently identified potent interferon (IFN)-γ producer. Indeed, IFN-γ was produced in those cultures, and pre-B cells lacking IFN-γ receptors, but not those lacking type I IFN receptors, were resistant to such an inhibition. Furthermore, even NK cells from mice lacking β2-microglobulin, which were known to be functionally dampened, inhibited pre-B cell proliferation as well. Thus, activated NK cells, which were expanded selectively by IL-15, could potentially regulate B lymphopoiesis through IFN-γ beyond the selection imposed upon self-recognition. [Copyright &y& Elsevier]

Published

2008

17. Bone marrow pre-B expansion by SL/Kh-Bomb1 locus: Not sufficient for lymphomagenesis

Author

Hiratsuka, Takuya, Tsuruyama, Tatsuaki, Kaszynski, Richard, Kometani, Kohei, Minato, Nagahiro, Nakamura, Takuro, Tamaki, Keiji, and Hiai, Hiroshi

Subjects

*BONE marrow, *IMMUNE system, *LYMPHOMAS, *LYMPHOPROLIFERATIVE disorders

Abstract

Abstract: The pre-B lymphoma in SL/Kh mice is a polygenic trait involving a number of host genes. In prelymphoma-stage bone marrow, transient pre-B cell expansion is induced by a host locus, Bomb1, and later followed by the emergence of a monoclonal population with a similar phenotype. To determine whether these pre-B cells represent precursors of lymphomas, we generated a congenic strain, NFS.SL/Kh-Bomb1 mice, by marker-assisted backcrossing to NFS. The congenic mice showed pre-B cell expansion, but pre-B lymphomas were not observed, even after 1 year of observation, irrespective of murine leukemia virus inoculation. Disturbed early B cell differentiation per se is not sufficient for SL/Kh lymphomagenesis. [Copyright &y& Elsevier]

Published

2008

18. Thymocytes, Pre-B Cells, and Organ Changes in a Mouse Model of Chronic Ethanol Ingestion—Absence of Subset-Specific Glucocorticoid-Induced Immune Cell Loss.

Author

Cook, Robert T., Schlueter, Annette J., Coleman, Ruth A., Tygrett, Lorraine, Ballas, Zuhair K., Jerrells, Thomas R., Nashelsky, Marcus B., Ray, Nancy B., Haugen, Thomas H., and Waldschmidt, Thomas J.

Subjects

*IMMUNODEFICIENCY, *IMMUNOLOGICAL deficiency syndromes, *ANTIGEN presenting cells, *ALCOHOL, *CORTICOSTERONE, *GLUCOCORTICOIDS, *B cells, *LYMPHOCYTES

Abstract

Background:  The well-known immune deficiency of the chronic alcoholic dictates the need for a long-term rodent ethanol administration model to evaluate the baseline immunologic effects of chronic ethanol abuse, and investigate the genetic determinants of those effects. Much published work with rodents has shown clearly that acute ethanol administration and short-term ethanol-containing liquid diets both cause elevated corticosterone and can cause significant thymocyte, pre-B cell and peripheral lymphocyte losses. Such losses may mask more subtle alterations in immune homeostasis, and in any case are generally short-lived compared with the span of chronic ethanol abuse. Thus, it is important to have a model in which long-term immune alterations can be studied free of corticosteroid-induced cell losses. Methods:  We have utilized chronic 20% (w/v) ethanol in water administration to several mouse strains for prolonged periods of time and evaluated serum corticosterone, immunologic stress parameters, and other organ changes by standard methods. Results:  We now confirm earlier reports that chronic ethanol in water administration to mice does not produce net elevations of corticosterone, although diurnal variation is altered. Importantly, there is neither selective loss of immune cell populations known to be corticosteroid sensitive, CD4+CD8+ thymocytes and pre-B cells, nor are changes observed in the histologic appearance of the thymus. Nonetheless, there are significant chronic ethanol effects in other tissues, including reduced heart weight, mild hepatic steatosis, alterations of gut flora, increased serum peptidoglycan, and as published elsewhere, immune system abnormalities. Conclusions:  This model of ethanol administration is convenient, sustainable for up to 1 year, demonstrably feasible in several mouse strains, permits good weight gains in most strains, and results in significant changes in a number of organs. The administration method also will permit modeling of long-term steady abuse punctuated by major binges, and is suitable for supplementation studies using water soluble additives. Overall, the method is useful for a wide range of studies requiring a chronic low-stress method of ethanol administration. [ABSTRACT FROM AUTHOR]

Published

2007

19. Dμ expression causes enrichment of MZ B cells, but is non permissive for B cell maturation in Rag2−/− mice even if combined with Bcl-2

Author

Wikström, Ingela, Bergqvist, Ingela, Holmberg, Dan, and Forssell, Johan

Subjects

*TRANSGENE expression, *B cells, *CELL receptors, *ANTIGEN presenting cells

Abstract

Abstract: Rearrangements in reading frame 2 promote the expression of a truncated heavy chain, the Dμ protein. Dμ can assemble into a pre-B cell receptor like complex that appears to induce a subset of signals elicited by full length μ, but cannot promote the pro-B to pre-B cell transition of Rag−/− B cells. In order to determine if this could stem from an impaired survival signal not properly induced by the Dμ protein, we introduced Bcl-2 into Dμ-transgenic, Rag2−/− mice. Despite the fact that the Bcl-2 transgene expression promoted some increase in the fraction of CD43− B cells, an identical increase was also observed in Rag2−/− mice. Moreover, whereas in μ-transgenic Rag2−/−Bcl-2+ mice, CD2 and CD25 expression were up regulated and c-Kit was down regulated, these markers were unaltered in Dμ-transgenic Rag2−/− Bcl-2+ mice compared to Rag2−/− Bcl-2+ mice, indicating that Dμ cannot support pre-B cell maturation despite extended survival of B cell precursors by Bcl-2. In addition, we observed that in Dμ-transgenic recombination competent mice, the Dμ induced partial block is permissive for marginal zone B cell development whereas the formation of follicular B cells is severely reduced. While the Dμ protein is expressed in peripheral B cells escaping the block, only a minor fraction of Dμ is exposed to the outer cell surface. [Copyright &y& Elsevier]

Published

2006

20. ZAP-70 upregulation in transformed B cells after early pre-BI cell transplant into NOD/SCID mice.

Author

Ruiz-Vela, Antonio, Piqueras, Raquel, Carvalho-Pinto, Carla, Gómez, Lucio, Yaniz-Galende, Elisa, Moreno-Ortiz, Mari Carmen, Bernad, Antonio, Harshman, Keith, and Martínez-A., Carlos

Subjects

*B cell differentiation, *MOUSE leukemia, *PRELEUKEMIA, *LEUCOCYTOSIS, *ANTIGEN presenting cells, *APOPTOSIS

Abstract

Understanding of the signal transduction pathways that lead to B cell development is of extreme interest to learn how alterations in these pathways might initiate malignant transformation. Long-term cultured early pre-BI cells can differentiate into IgM+ B cells after transplant into NOD/SCID mice, offering the possibility to explore checkpoints in B cell development. Using DNA microarray and Western blot analysis of IgM+ B cells vs parental early pre-BI cells, we demonstrated that zeta-associated protein 70 (ZAP-70) is upregulated in our B cell differentiation model. Unlike parental ZAP-70− early pre-BI cells, ZAP-70+ IgM+ B cells exhibited a transformed phenotype, as indicated by BCL-6 expression, a high Ki-67 proliferation index, resistance to IL-7 deprivation-induced apoptosis, and an increased repopulation rate in NOD/SCID mice. These data show the characterization and generation of a novel murine leukemia model with many similarities to human ZAP-70+ B cell chronic lymphocytic leukemia.Oncogene (2005) 24, 5119–5124. doi:10.1038/sj.onc.1208706; published online 18 April 2005 [ABSTRACT FROM AUTHOR]

Published

2005

21. Pre-B cell loss in senescence coincides with preferential development of immature B cells characterized by partial activation and altered Vh repertoire

Author

Wilson, Emily L., King, Anne M., Sherwood, Erin M., and Riley, Richard L.

Subjects

*B cells, *LYMPHOCYTES, *GENOTYPE-environment interaction, *CELL death, *MICE

Abstract

Abstract: Senescent mice show decline in B lymphopoiesis marked by reduced pre-B cells. Analysis of bone marrow from aged (∼2 years old) BALB/c mice indicates that, in senescence, an increased proportion of immature B cells exhibit a CD43/S7+ surface phenotype. This results from continued production of new CD43/S7+ B cells in aged mice from their limited pre-B cell pool while production of CD43/S7- immature B cells is highly reduced. CD43/S7 is ordinarily observed on a minor subset of immature B cells in young mice and is indicative of their partial activation. Senescent immature B cells, both ex vivo and derived in vitro, also demonstrate increased expression of VhS107 concomitant with CD43/S7. These alterations in the phenotype and Vh repertoire among senescent immature B cells likely originate prior to surface Ig expression. In aged mice with depleted pre-B and immature B cells in vivo, pre-B and immature B cells exhibited increased apoptosis in vitro. Dexamethasone-induced apoptosis among B lineage cells in young adult mice also resulted in pre-B cell loss and increased expression of CD43/S7 and VhS107 among immature B cells similar to that observed spontaneously in aged mice. These results suggest that old age, possibly due to increased apoptosis, results in loss of pre-B cells and alterations in the phenotype and Vh repertoire of newly derived B cells. [Copyright &y& Elsevier]

Published

2005

22. Quantification of Jκ signal end breaks in developing B cells by blunt-end linker ligation and qPCR

Author

Curry, John D., Li, Lydia, and Schlissel, Mark S.

Subjects

*DNA, *BONE marrow, *LYMPHOCYTES, *CELL culture

Abstract

Abstract: Introduction of a double-strand DNA break at the junction between a rearranging gene segment and its flanking recombination signal sequence (RSS) is the first step of V(D)J recombination. Such DNA breaks can be detected by either Southern blot hybridization or ligation-mediated PCR. While Southern blotting is easily quantifiable, it is often insufficiently sensitive and while LM-PCR is far more sensitive, it is poorly quantifiable. Reported here is a LM-qPCR assay which relies on real-time qPCR to provide an absolute measure of recombinase-mediated, or any other specific, double-strand DNA break in genomic DNA. The efficiency of the initial ligation reaction was found to be relatively low with just 3% of potential targets undergoing linker ligation. Using this assay, approximately 16% of murine bone marrow pre-B cells were determined to contain a dsDNA break adjacent to the Jκ1 gene segment. In addition, the kinetics of JΚκ1 dsDNA breaks in a temperature-sensitive cell line induced to recombine its κ locus was determined. [Copyright &y& Elsevier]

Published

2005

23. Interleukin-7 induces apoptosis of 697 pre-B cells expressing dominant-negative forms of STAT5: evidence for caspase-dependent and -independent mechanisms.

Author

Lanvin, Olivia, Mullié, Catherine, Mazière, Cécile, Fuentes, Vincent, Bissac, Eliane, Dantin, Françoise, Mazière, Jean-Claude, Régnier, Aline, Lassoued, Kaiss, Gouilleux-Gruart, Valérie, and Gouilleux, Fabrice

Subjects

*INTERLEUKINS, *APOPTOSIS, *B cells, *CYTOKINES, *TRANSCRIPTION factors

Abstract

The transcription factors STAT5A and STAT5B (STAT: signal transducer and activator of transcription) play a major role in the signaling events elicited by a number of growth factor and cytokine receptors. In this work, we aimed to investigate the role of STAT5 in human precursor B cell survival by introducing dominant-negative (DN) forms of STAT5A or STAT5B in the 697 pre-B cell line. All clones expressing DN forms of either transcription factor exhibited a higher spontaneous apoptotic rate that was massively enhanced upon interleukin-7 (IL-7) stimulation. This was associated with caspase 8 cleavage, mitochondrial transmembrane potential disruption and caspase 3 activation. However, the DN forms of STAT5 did not alter the expression of Bcl-2, Bax, Bcl-x, Bim, A1 and Mcl1 proteins in IL-7-stimulated cells. The pancaspase inhibitor Z-Val-Ala-Asp-fluoromylmethyl ketone partially suppressed IL-7-mediated mitochondrial transmembrane potential disruption and cell death, suggesting that IL-7 induced the death of DN STAT5 expressing 697 cells through caspase-dependent and -independent mechanisms that both require mitochondrial activation.Oncogene (2004) 23, 3040-3047. doi:10.1038/sj.onc.1207450 Published online 29 March 2004 [ABSTRACT FROM AUTHOR]

Published

2004

24. Aged mice exhibit distinct B cell precursor phenotypes differing in activation, proliferation and apoptosis

Author

Van der Put, Elaine, Sherwood, Erin M., Blomberg, Bonnie B., and Riley, Richard L.

Subjects

*AGING, *BONE marrow, *B cells, *PHENOTYPES

Abstract

Senescence in murine models is associated with a reduction, albeit heterogeneous, in bone marrow pre-B cells. We have categorized aged BALB/c mice into two phenotypes based on their patterns of pre-B/pro-B cell loss. Each phenotype is characterized by distinct responses to the growth cytokine IL-7 and capacity for survival in vitro. A ‘moderate’ loss of late-stage pre-B cells (25–80%) coincided with decline in proliferation to rmIL-7. This was also associated with a decrease in the frequency of pro-B cells which increased phosphotyrosine content upon IL-7 stimulation, an indicator of early activation events. A ‘severe’ loss of pre-B cells (>80%) resulted in a reduced pro-B cell pool which retained normal activation and proliferative responses to IL-7. B cell precursors from aged mice with severe alterations in B lymphopoiesis displayed increased susceptibility to apoptosis in comparison to both aged mice with moderate B cell precursor loss and young mice. Conceivably, during senescence, aged mice may initially accumulate B cell precursors which are poorly responsive to IL-7. Progressively, these refractory B cell precursors may be eliminated via apoptosis; however, the remaining limited pool of B cell precursors retains the capacity to respond to IL-7 stimulation. [Copyright &y& Elsevier]

Published

2003

25. Biological Characterization of 8-Cyclopropyl-2-(pyridin-3-yl)thiazolo[5,4

Author

Corinne, Fruit, Florence, Couly, Rahul, Bhansali, Malini, Rammohan, Mattias F, Lindberg, John D, Crispino, Laurent, Meijer, and Thierry, Besson

Subjects

DYRK family kinases, thiazolo[5,4-f]quinazolin-9(8H)-one, CMGC kinases, Communication, pre-B cells, quiescence, SH-SY5Y-Tau-4R cells

Abstract

Dual-specificity tyrosine phosphorylation-regulated kinases (DYRKs) hyperactivity has been linked to the development of a number of human malignancies. DYRK1A is the most studied family member, and the discovery of novel specific inhibitors is attracting considerable interest. The 8-cyclopropyl-2(pyridin-3-yl)thiazolo[5,4-f]quinazolin-9(8H)-one (also called FC162) was found to be a promising inhibitor of DYRK1A and was characterized in biological experiments, by western transfer and flow cytometry on SH-SY5Y and pre-B cells. Here, the results obtained with FC162 are compared to well-characterized known DYRK1A inhibitors (e.g., Leucettine L41 and EHT1610).

Published

2019

26. Biological Characterization of 8-Cyclopropyl-2-(pyridin-3-yl)thiazolo[5,4-f]quinazolin-9(8H)-one, a Promising Inhibitor of DYRK1A

Author

Mattias F. Lindberg, Malini Rammohan, John D. Crispino, Corinne Fruit, Florence Couly, Rahul S. Bhansali, Thierry Besson, Laurent Meijer, Chimie Organique et Bioorganique : Réactivité et Analyse (COBRA), Institut Normand de Chimie Moléculaire Médicinale et Macromoléculaire (INC3M), Institut de Chimie du CNRS (INC)-École Nationale Supérieure d'Ingénieurs de Caen (ENSICAEN), Normandie Université (NU)-Normandie Université (NU)-Institut national des sciences appliquées Rouen Normandie (INSA Rouen Normandie), Institut National des Sciences Appliquées (INSA)-Normandie Université (NU)-Institut National des Sciences Appliquées (INSA)-Université Le Havre Normandie (ULH), Normandie Université (NU)-Université de Rouen Normandie (UNIROUEN), Normandie Université (NU)-Centre National de la Recherche Scientifique (CNRS)-Université de Caen Normandie (UNICAEN), Normandie Université (NU)-Institut de Chimie du CNRS (INC)-École Nationale Supérieure d'Ingénieurs de Caen (ENSICAEN), Normandie Université (NU)-Centre National de la Recherche Scientifique (CNRS)-Institut de Chimie Organique Fine (IRCOF), Université de Rouen Normandie (UNIROUEN), Institut National des Sciences Appliquées (INSA)-Normandie Université (NU)-Institut National des Sciences Appliquées (INSA)-Centre National de la Recherche Scientifique (CNRS)-Centre National de la Recherche Scientifique (CNRS), The University of Chicago Medicine [Chicago], ManRos Therapeutics, and Northwestern University Feinberg School of Medicine

Subjects

DYRK1A, pre-B cells, Pharmaceutical Science, SH-SY5Y-Tau-4R cells, Pre-B-Cells, 01 natural sciences, Flow cytometry, 03 medical and health sciences, Drug Discovery, medicine, [CHIM]Chemical Sciences, quiescence, Tyrosine, 030304 developmental biology, DYRK family kinases, 0303 health sciences, thiazolo[5, medicine.diagnostic_test, 010405 organic chemistry, Chemistry, Kinase, 4-f]quinazolin-9(8H)-one, 0104 chemical sciences, 3. Good health, Family member, Leucettine L41, Biochemistry, CMGC kinases, Molecular Medicine

Abstract

International audience; Dual-specificity tyrosine phosphorylation-regulated kinases (DYRKs) hyperactivity has been linked to the development of a number of human malignancies. DYRK1A is the most studied family member, and the discovery of novel specific inhibitors is attracting considerable interest. The 8-cyclopropyl-2(pyridin-3-yl)thiazolo[5,4-f]quinazolin-9(8H)-one (also called FC162) was found to be a promising inhibitor of DYRK1A and was characterized in biological experiments, by western transfer and flow cytometry on SH-SY5Y and pre-B cells. Here, the results obtained with FC162 are compared to well-characterized known DYRK1A inhibitors (e.g., Leucettine L41 and EHT1610).

Published

2019

27. IL-7 sensitizes human pre-B cells but not pro-B cells to Fas/APO-1 (CD95)-mediated apoptosis.

Author

Levy, Y., Benlagha, K., Buzyn, A., Colombel, M., Brouet, J.-C., and Lassoued, K.

Subjects

*B cells, *APOPTOSIS, *HOMEOSTASIS, *ANTIGENS, *MOLECULES, *LYMPHOCYTES

Abstract

Homeostasis of human B cell development is maintained by a complex network of cytoplasmic and surface expressed molecules. Abnormalities in this process may result in the expansion of malignant B cell precursors in B lineage acute lymphoblastic leukaemia (ALL). ALL cells share surface antigens with normal early precursor B cells. We have studied here the role of Fas/APO-1 (CD95) antigen on leukaemic precursor B cell line growth and survival, and the modulation of its effects by signals involved in normal early B cell development. Four ALL cell lines representative of the early steps of B cell differentiation are shown to express surface Fas/APO-1 (CD95) antigen and to undergo apoptosis in the presence of anti-Fas cross-linking antibodies. This effect is strongly enhanced when pre-B, but not pro-B cells, are pretreated with IL-7 but not with IL-2, IL-3, IL-4 or IL-10. Furthermore, pre B cell death induced by anti-Fas antibodies in combination with IL-7 is increased upon pre B receptor but not CDI9 cross-linking. Bcl-2 and Bax protein expression is not influenced by IL-7 or pre-BR stimulation in either pro-B or pre-B cell lines. These results indicate that signals involved in normal early B cell development can modulate the Fas (CD95)-mediated apoptosis of leukaemic precursor B cells. [ABSTRACT FROM AUTHOR]

Published

1997

28. Effects of ethanol consumption and withdrawal on B cell subpopulations in murine bone marrow.

Author

Kruger, T. W. and Jerrells, T. R.

Subjects

*ALCOHOL, *BONE marrow, *LYMPHOCYTES, *IMMUNE system, *CYTOLOGY, *CELL proliferation, *RODENTS

Abstract

We designed studies to examine the effects of ethanol consumption and withdrawal on the numbers of pre-B and B cells in murine bone marrow. Flow cytometric analysis of B220 and surface IgM expression on bone marrow cells revealed that consumption of ethanol by mice for 7 days led to a significant reduction in pre-B cells. The number of mature B cells in the bone marrow of these animals, however, did not differ from that of control mice. In contrast, examination of bone marrow obtained from mice at various times after withdrawal from ethanol showed significantly fewer numbers of mature B cells and an even greater toss of pre-B cells. This effect was seen for relatively long periods after withdrawal. These study findings are interpreted to suggest that ethanol consumption results in changes in the pre-B cell population in murine bone marrow. It also appears that withdrawal from ethanol results in more profound changes in the mature B cell population of the bone marrow than those that occur during ethanol consumption. [ABSTRACT FROM AUTHOR]

Published

1994

29. Overexpression of Bcl-2 does not rescue impaired B lymphopoiesis in IL-7 receptor-deficient mice but can enhance survival of mature B cells.

Author

Maraskovsky, E, Peschon, JJ, McKenna, H, Teepe, M, and Strasser, A

Abstract

IL-7 receptor-deficient (IL-7R-/-) mice are lymphopenic as a result of defective cell production at early steps in both B and T lymphopoiesis. In the bone marrow, there is an incomplete block in B cell development at the transition from the pro-B to the pre-B cell stage. As a consequence, peripheral lymphoid organs of IL-7R-/- mice contain abnormally low numbers of mature surface (s) Ig-expressing B cells and this is accompanied by a relative increase in immature sig- B cells. Transgenic expression of the anti-apoptotic protein Bcl-2 in IL-7R-/- mice rescues the defect in T cell development and in mature T cell function. The present report shows that constitutive expression of Bcl-2 is incapable of rescuing B lymphopoiesis in IL-7R-/- mice but can enhance survival of those mature B cells which escape the developmental arrest. Thus the essential role of IL-7R signaling in B lymphoid cells cannot be replaced by Bcl-2, indicating that in B lymphopoiesis IL-7R signaling is necessary for promoting cell division and/or for inhibiting a Bcl-2-insensitive pathway to apoptosis. [ABSTRACT FROM PUBLISHER]

Published

1998

30. Expression of Vpre-B3 (8HS-20) molecules by alternative RNA processing.

Author

Shinji Haglwara, Yasuko Tsunetsugu-Yokota, Hiroshi Kimoto, and Toshitada Takemori

Abstract

In pre-B cells, μchains are expressed in association with ‘surrogate’ L chains encoded by the λ5 and Vpre-B1 genes. In addition to their association with λ5 and Vpre-B1, μ chains in pre-B cells are associated with the products of the Vpre-B3 gene (formerly designated 8HS-20), which display a distinct association withμ chains and biochemical properties in terms of mol. wt, plvalue and glycosylatlon. However, the mechanism of the generation of Vpre-B3 isoforms has been unknown. The present study Indicates that the Vpre-B3 gene transcript underwent alternative RNA processing In normal B cells, In a pre-B cell lymphoma and in a mature B cell lymphoma, WEHI 231, that was transfected with the Vpre-B3genomic clone. Vpre-B3 isoforms were expressed In a WEHI 231 cell line transfected with the Vpre-B3ad genomic clone, comparable In biochemical nature to those expressed In a pre-B cell lymphoma. In contrast, expression of one of the isoforms was missing In a cell line transfected with the Vpre-B3 cDNA clone. These results suggest that Vpre-B3 isoforms with distinct biochemical characteristics are derived from alternatively processed Vpre-B3 mRNA. [ABSTRACT FROM AUTHOR]

Published

1996

31. Measurement of recombinase activity in a set of related Abelson murine leukemic virus pre-B cell lines: DJ/DJ lines have more recombinase activity than do VDJ/VDJ lines.

Author

Eisen, Andrea F., Atkinson, Michael J., Celler, Jakub W., Paige, Christopher J., and Wu, Gillian E.

Abstract

The VDJ recombination potential of a number of Abelson murine leukemic virus transformed fetal liver cell lines derived from (C57BL/6 × BALB/c) F1 mice was measured. The specific developmental stage of each line was determined using Southern blot anlaysis to ascertain their rearrangement status at the immunoglobulin heavy chain locus (DJ/DJ, VDJ/DJ or VDJ/VDJ). It was observed that DNA from DJ/DJ lines gave many more ‘subhaploid’ bands hybridizing with JH than did DNA from VDJ/VDJ lines. While the lack of appropriate substrate (VDJ/VDJ lines have exhausted the normal IgH substrate) contributes to the decrease In ‘subhaploid bands1, this result Indicates that the rate of ongoing immunoglobulin heavy chain gene rearrangement was higher in the DJ/DJ lines. However, when the lines were examined using the assay developed by Hesse et al. (4) to measure VDJ recombinase activity, it was found that although all lines had recombinase activity, the DJ/DJ lines had four times more VDJ recomblnase activity than did the VDJ/VDJ lines. [ABSTRACT FROM PUBLISHER]

Published

1991

32. Signal transmission through the B cell-specific MB-1 molecule at the pre-B cell stage.

Author

Nomura, Jun, Matsuo, Tatsuya, Kubota, Eiro, Kimoto, Masao, and Sakaguchi, Nobuo

Abstract

Specific binding of antigens to the surface immunoglobulln M (slgM) triggers B cells with several biochemical events Involved in receptor-mediated signal transmission for proliferation and differentiation into antibody-producing cells. Recent studies with the Digitonin lysis method identified the slgM-assoclated component, IgM-α (B34)/lg-β, as the possible candidate for the transducer molecule(s) In the immunoglobulln receptor-mediated signal transmission. The 34 kdprotein (B34 or IgM-α) of this component Is suggested to be encoded by the B cell-specific mb-1 gene. We prepared monoclonal antibodies which recognize the mb-1 gene product (MB-1) and studied the functional role of MB-1 In the signal transmission In B lineage cells. Using murine pre-B lymphoma cells (18–81 and 70Z/3), we demonstrated the early phase increase of the Intracellular [Ca] concentration and the subsequent inhibition of the proliferation by the monoclonal anti-MB-1 antibody (11–18–5). These results clearly demonstrate signal transmission through the surface MB-1 molecule on B lineage lymphomas. This MB-1-mediated signal transmission in pre-B cell lines would suggest an alternative function of MB-1 acting at the pre-B cell stage. [ABSTRACT FROM PUBLISHER]

Published

1991

33. Defining the immune mechanism with monoclonal antibodies.

Author

Klinman, Norman, Denis, Kathleen, and Sherman, Linda

Abstract

It has long been realized that only the study of homogeneous antibodies or cell populations could enable a definitive understanding of much of the immune mechanism. Hybridoma technology has greatly facilitated such approaches. Hybridoma antibodies have been used to delineate both B cell and T cell subpopulations. T cell studies per se have been accomplished by the use of T cell hybridoma cell lines producing a variety of factors. Anti-idiotypes against B cell hybridoma antibodies have been used to characterize T cell receptors and factors. B cell studies have been facilitated by hybridomas that have made available the immunoglobulin of pre-B cells or defective B cell lines. Hybridoma antibodies have also been used to dissect closely related antibody families and the potential for responsiveness against a variety of antigenic determinants. Finally, hybridomas have provided a primary source of material for protein and DNA sequence analysis. In our laboratories hybridoma antibodies derived against the murine H-2 locus have demonstrated the ability of B cell antibodies to discriminate amongst H2 mutants-a capacity previously attributed only to T cell specificities. Hybridoma antibodies have also been generated by fusions with antigen stimulated neonatal B cells to provide homogeneous antibodies reflective of the earliest developmental immunoglobulin readout. Such probes should increase our understanding of the processes involved in the generation of both the T and B cell repertoires. [ABSTRACT FROM AUTHOR]

Published

1981

34. Full length RAG2 expression enhances the DNA damage response in pre-B cells.

Author

Byrum, Jennifer N., Hoolehan, Walker E., Simpson, Destiny A., Rodgers, William, and Rodgers, Karla K.

Subjects

*DOUBLE-strand DNA breaks, *DNA damage, *DNA repair, *CELL cycle, *CASPASES

Abstract

V(D)J recombination by the RAG1 and RAG2 protein complex in developing lymphocytes includes DNA double strand break (DSB) intermediates. RAG2 undergoes export from the nucleus and enrichment at the centrosome minutes following production of DSBs by genotoxic stress, suggesting that RAG2 participates in cellular responses to DSBs such as those generated during V(D)J recombination. To determine the effect of RAG2 expression on cell viability following DSB generation, we measured pre-B cells that expressed either full length (FL) wild-type RAG2, or a T490A mutant of RAG2 that has increased stability and fails to undergo nuclear export following generation of DSBs. Each RAG2 construct was labeled with GFP at the N-terminus. Compared to the T490A mutant, cells expressing FL RAG2 exhibited elevated apoptosis by 24 h following irradiation, and this coincided with a greater amount of Caspase 3 cleavage measured in cell lysates. Pre-B cells expressing either RAG2 protein exhibited similar increases in phospho-p53 levels following irradiation. Interestingly, FL RAG2-expressing cells exhibited elevated division relative to the T490A clone beginning ~24 h following irradiation, as well as an increased percentage of cells proceeding through mitosis, suggesting an improved rate of recovery following the initial burst in apoptosis. Altogether, these data show that FL RAG2, but not its stable nuclear export-defective T490A mutant, participates in pre-B cell decisions between apoptosis versus DNA repair and cell cycle progression following DNA damage. [ABSTRACT FROM AUTHOR]

Published

2021

35. Biological Characterization of 8-Cyclopropyl-2-(pyridin-3-yl)thiazolo[5,4-f]quinazolin-9(8H)-one, a Promising Inhibitor of DYRK1A.

Author

Fruit, Corinne, Couly, Florence, Bhansali, Rahul, Rammohan, Malini, Lindberg, Mattias F., Crispino, John D., Meijer, Laurent, and Besson, Thierry

Subjects

*KINASES, *FLOW cytometry, *TYROSINE

Abstract

Dual-specificity tyrosine phosphorylation-regulated kinases (DYRKs) hyperactivity has been linked to the development of a number of human malignancies. DYRK1A is the most studied family member, and the discovery of novel specific inhibitors is attracting considerable interest. The 8-cyclopropyl-2(pyridin-3-yl)thiazolo[5,4-f]quinazolin-9(8H)-one (also called FC162) was found to be a promising inhibitor of DYRK1A and was characterized in biological experiments, by western transfer and flow cytometry on SH-SY5Y and pre-B cells. Here, the results obtained with FC162 are compared to well-characterized known DYRK1A inhibitors (e.g., Leucettine L41 and EHT1610). [ABSTRACT FROM AUTHOR]

Published

2019

36. RAG-Mediated DNA Breaks Attenuate PU.1 Activity in Early B Cells through Activation of a SPIC-BCLAF1 Complex.

Author

Soodgupta, Deepti, White, Lynn S., Yang, Wei, Johnston, Rachel, Andrews, Jared M., Kohyama, Masako, Murphy, Kenneth M., Mosammaparast, Nima, Payton, Jacqueline E., and Bednarski, Jeffrey J.

Abstract

Early B cell development is regulated by stage-specific transcription factors. PU.1, an ETS-family transcription factor, is essential for coordination of early B cell maturation and immunoglobulin gene (Ig) rearrangement. Here we show that RAG DNA double-strand breaks (DSBs) generated during Ig light chain gene (Igl) rearrangement in pre-B cells induce global changes in PU.1 chromatin binding. RAG DSBs activate a SPIC/BCLAF1 transcription factor complex that displaces PU.1 throughout the genome and regulates broad transcriptional changes. SPIC recruits BCLAF1 to gene-regulatory elements that control expression of key B cell developmental genes. The SPIC/BCLAF1 complex suppresses expression of the SYK tyrosine kinase and enforces the transition from large to small pre-B cells. These studies reveal that RAG DSBs direct genome-wide changes in ETS transcription factor activity to promote early B cell development. • RAG DNA breaks upregulate SPIC, which induces genome-wide changes in PU.1 activity • SPIC binds to gene-regulatory elements, resulting in loss of PU.1 at these regions • SPIC complexes with BCLAF1 to suppress transcription in response to RAG DNA breaks • SPIC/BCLAF1 inhibits SYK and promotes transition from large to small pre-B cells ETS-family transcription factors are key regulators of early B cell development. Soodgupta et al. show that RAG-induced DNA breaks generated during antigen receptor gene recombination activate a SPIC/BCLAF1 transcription factor complex that counters PU.1 activity and regulates gene expression changes to promote transition from large to small pre-B cells. [ABSTRACT FROM AUTHOR]

Published

2019

37. EFFECTS OF A COUMESTAN DERIVATIVE AND CUCURBITACIN B ON APOPTOSIS OF PRE-B CELLS.

Author

Costuleanu, Marcel, Iancu, Roxana Irina, Toader, Ştefan, Amititeloaie, Carmen, and Vasincu, Decebal

Subjects

*APOPTOSIS, *CYCLOSPORINE, *CELLS, *LYMPHOCYTES

Abstract

One of the suggested pharmacologic mechanisms for antitumoral effects of coumestan and cucurbitacin B derivatives might be represented by the modulation of apoptosis through mitochondrial and cytosolic calcium fluxes. Thus, the goal of our studies (each in triplicate) was represented by the characterization of the effects of 7-methoxy-5,11,12-trihydroxy-coumestan, an inhibitor of NF-kappa B-mediated transcription, and of cucurbitacin B hydrate, an inhibitor of signaling mediated by JAK, on pre-B cells apoptosis, using contrast microscopy. Cyclosporine A (1 μM) alone did not induce statistical significant apoptotic effects on murine pre-B cells (8.12±1.97%). For some experiments, pre-B lymphocytes were treated with 5 μM 7-methoxy-5,11,12-trihydroxy-coumestan in culture medium for 48 hours. As proven, 91.39±7.47% of the pre-B cells are not going apoptotic after 48 h (statistically not significant results, p>0.05) in the presence of cyclosporine A (1 μM). On the other hand, 5 μM cucurbitacin B hydrate induced a statistically significant apoptosis (62.95±5.99, p<0.05) in pre-B lymphocytes after 48 h of treatment in the presence of cyclosporine A (1 μM). The fine mechanisms need deeper exploration starting from the point that cyclosporine A concomitant administration did not block the effects of cucurbitacin B hydrate, a very similar structural compound to cucurbitacin I. [ABSTRACT FROM AUTHOR]

Published

2019

38. Defining cell-surface antigenic markers for mouse T and B cells

Author

Martin Raff

Subjects

lcsh:Immunologic diseases. Allergy, carrier effect, Ig, Lymphocyte, Population, Immunology, pre-B cells, T cells, Spleen, Biology, Immune system, Antigen, medicine, Immunology and Allergy, education, Lymph node, thy1, education.field_of_study, B cells, cell-surface markers, medicine.anatomical_structure, Lymphatic system, biology.protein, Antibody, lcsh:RC581-607

Abstract

I began my scientific career in October 1968 at the National Institute for Medical Research (NIMR) in London. I was 30-years old, having just finished my training in clinical neurology in Boston, and I had come to work with Avrion (Av) Mitchison. I had much to learn, as I had done no basic research and knew very little about immunology. It was an exciting time – both in immunology and at the NIMR. There was increasing evidence that there were two types of lymphocytes, T and B cells, responsible for adaptive immune responses but there were no good ways to distinguish or separate them. Av had recently heard the Boston immunologist Arnold Reif describe a mouse isoantigen called theta (θ), which was present in the brain and on the surface of thymocytes (1, 2). Av wondered if θ might be present on T but not B cells, in which case it could serve as a useful cell-surface marker for mouse T cells. He gave me the relevant Reif papers, an aliquot of a mouse anti-θ antiserum that he had begun making, and set me free. In a commentary written in 2008 for the Pillars of Immunology series in the Journal of Immunology (3), the Seattle immunologist Pamela Fink colorfully described what happened next. Here, I give an abbreviated account of this history but broaden it to include the fortuitous finding that immunoglobulin (Ig) can serve as a cell-surface marker for B cells. To detect θ on mouse lymphocytes, I first used an antibody- and complement-dependent 51chromium-release cytotoxicity assay, which I learned from my lab-mate Marion Ruskowicz (4). I found that the antiserum and complement killed essentially all thymus lymphocytes but only a subset of lymph node and spleen lymphocytes. To test whether the θ-positive lymphocytes in lymph node and spleen were T cells, I analyzed cells from pathogen-free mice that had been treated since birth with a rabbit antiserum made against mouse thymocytes (5) and were therefore T-cell-depleted; Sandra Nehlson, a Ph.D. student with Peter Medawar who worked across the hall, generously provided these mice. I found that the spleen and lymph nodes of the mice contained normal numbers of θ-negative lymphocytes but greatly reduced numbers of θ-positive lymphocytes, strongly suggesting that Av’s hunch was right – θ is present on T but not B cells (6). Schlesinger and Yron independently published very similar findings around the same time (7); unfairly, their paper received far less attention, probably because its title lacked the punch line of their findings. Later, in collaboration with Henry Wortis, who worked next door, we confirmed these findings in other T-cell-deficient mice, including congenitally athymic nude mice (8). I then tested the functional properties of θ-positive spleen cells by analyzing the cells involved in an adoptive cell-transfer system that Av had developed to study the cooperation between two populations of spleen cells – one from mice immunized with a hapten (NIP) coupled to a carrier protein (chicken γ-globulin, CGG) and another from mice immunized with an uncoupled, second carrier protein (bovine serum albumin, BSA). He had shown that, when both cell populations, but not either one alone, are transferred into a sub-lethally irradiated mouse, the recipient mouse produces large amounts of anti-NIP antibodies in the blood when immunized with NIP-BSA but not with NIP-CGG – an example of the so-called carrier effect (9). In my experiments, before transferring the cells, I treated one or other population with anti-θ antibodies and complement to kill the T cells, using normal mouse serum plus complement as a control. In this way, I could show that the relevant cells in the BSA-immunized population were T cells, whereas the relevant cells in the NIP-CGG-immunized population, which produced the anti-NIP antibodies (9), were not (10). This experiment provided direct evidence that T cells recognizing antigenic determinants on a protein can help B cells make antibodies against different antigenic determinants on the same protein (11). It also established the value of antibodies that recognize cell-type-specific surface antigens, which rapidly became standard tools in immunology and, later, in various other branches of biology. Remarkably, Av declined to put his name on these two Nature papers (6, 10), even though the projects were his idea and he had begun to produce anti-θ antibodies before I arrived in London. This exceptional generosity had an enormous influence on my career. Theta (now called Thy-1) rapidly became a standard marker for mouse T cells, and the two single-author Nature papers gave me immediate international recognition, after only 2 years doing basic science. Nonetheless, if I had known then what I know now, I would have insisted that Av’s name was on the papers, to indicate his crucial contributions to the work. Av always did his own experiments and made many landmark contributions to immunology; because he usually allowed his students and postdoctoral fellows to publish on their own, however, his actual contributions are far greater than are documented in the literature. To visualize θ directly on the surface of living T cells, I turned from cytotoxicity assays to immunofluorescence experiments. In these experiments, I visualized the bound mouse anti-θ antibodies using fluorescent rabbit anti-mouse-Ig antibodies. A surprise came from control experiments in which I omitted the anti-θ antibodies and found that the fluorescent anti-Ig antibodies on their own labeled a substantial proportion of lymphocytes in cell suspensions prepared from various peripheral lymphoid organs, although not in suspensions of thymocytes. Roger Taylor, working across the hall with Michel Sternberg, had independently obtained similar results using radiolabeled anti-mouse-Ig antibodies, and we published our findings together (12). Although a number of immunologists, including Av, had suspected that the antigen receptors on lymphocytes might be Ig proteins, ours was one of the first direct demonstrations of Ig molecules on the surface of lymphocytes. The finding of Ig on some peripheral lymphocytes but not others raised the question of which class of lymphocyte expressed the cell-surface Ig. To find out, I studied lymphocytes from normal mice and from various T-cell-depleted mice, labeling the cells with anti-mouse-Ig antibodies, with or without first labeling them with mouse anti-θ antibodies. The results were unambiguous: the Ig-positive cells were θ-negative, implying that they were B cells, whereas the θ-positive T cells were Ig-negative (13). (The analysis was greatly helped by the fact that the Ig was distributed in a cap at one pole of the B cells, whereas θ was distributed as a ring on the T cells; later, Stefanello de Petris and I, and Roger Taylor and Phillip Duffus independently, showed that the binding of the anti-Ig antibodies induces the B cells to actively redistribute their surface Ig molecules into a cap (14) – but that is another story.) The Journal of Experimental Medicine rejected my paper as not being sufficiently interesting, and it was published in Immunology, a low impact journal. Despite this (and its unhelpful title), it became a Citation Classic (15), which taught me an important lesson: it is what you publish rather than where you publish it that matters most. The finding of Ig on the surface of B cells but not T cells led to a prolonged and frustrating search by many laboratories for the antigen receptors on T cells, which were only identified as distinct Ig-like proteins years later, after a number of false leads (16). Cell-surface Ig became a standard marker for B cells in all vertebrates. When I moved with Av to University College London, for example, John Owen and I collaborated with Max Cooper (who was on sabbatical from the University of Alabama) and used anti-Ig antibodies and explant cultures to study the development of B cells. We showed that mouse B cells develop in the fetal liver and adult bone marrow (17), rather than in gut-associated lymphoid tissues as had been proposed by Max and others. We later used Max’s class-specific anti-Ig antibodies to demonstrate that the B cells arise from pre-B cells, which have already begun to make IgM heavy chains (18). Remarkably, these first few years in science were the most productive in my research career. This early success was largely the result of good luck: I was at the right place at the right time, with a generous and inspiring mentor. And it was why I became a scientist rather than a practicing neurologist.

Published

2014

39. Human pre-B cell receptor signal transduction: evidence for distinct roles of PI3kinase and MAP-kinase signalling pathways

Author

Kolandaswamy, Anbazhagan, Amrathlal, Rabbind Singh, Piec, Isabelle, Ibata, Stella, Alleaume-De Martel, Céline, Eliane, Bissac, Brassart, Bertrand, Nyga, Rémy, Taylor, Naomi, Fuentes, Vincent, Jacques, Rochette, and Kaïss, Lassoued

Subjects

receptor signalling, hemic and lymphatic diseases, pre-B cells, pre-BCR, MAPK, PI3K, Original Research

Abstract

Pre-BCR acts as a critical checkpoint in B cell development. However, its signalling cascade still remains indistinctly characterised in human. We investigated pre-BCR signalling pathway to examine its regulation in normal primary pre-B lymphocytes and pre-B cell lines. In cell lines, early signalling events occurring after pre-BCR stimulation include phosphorylation of Lyn, Blk and Syk together with ZAP70, Btk, Vav, PLC-γ2 and various adaptor proteins, such as BLNK, LAB, LAT and SLP-76. Further downstream, these molecules induced activation of the PI3K/AKT and MAP-kinase resulting in an augmentation of canonical NF-κB pathways and cFos/AP1 activation. PI3K and MAPK exerted opposing effects on the pre-BCR-induced activation of the canonical NF-κB and c-Fos/AP1 pathways. Immediate nuclear export of FoxO3A and delayed import of IRF4 were additional events observed after pre-BCR crosslinking in primary cells. Pre-BCR-induced down-regulation of Rag1, Rag2, E2A and Pax5 transcripts occurred in a PI3K-dependent manner. Finally we bring evidence that pre-BCR stimulation or co stimulation with CD19 enhances cell cycle signal.

Published

2013

40. The Presence of Precursors of Benign Pre-B Lymphoblasts (Hematogones) in the Bone Marrow of a Paediatric Patient with Cytomegalovirus Infection

Author

José Uberos, P Jiménez-Gámiz, M Díaz-Molina, Francisco Moreno-Madrid, A Ramírez-Arredondo, Antonio Molina-Carballo, [Moreno-Madrid,F, Ramírez-Arredondo,A] Servicio de Pediatría, Ciudad Sanitaria Virgen de las Nieves. [Uberos,J, and Molina-Carballo A] Distrito Sanitario Granada. [Jiménez-Gámiz,P] Servicio de Hematología, Ciudad Sanitaria Virgen de las Nieves, Granada , Spain.

Subjects

Pathology, medicine.medical_specialty, Diseases::Neoplasms::Neoplasms by Histologic Type::Leukemia [Medical Subject Headings], pre-B cells, Congenital cytomegalovirus infection, Cytomegalovirus, Case Report, acute lymphoblastic leukemia, Acute lymphoblastic leukemia, Hematogones, lcsh:RC254-282, Pre-B cells, Immunophenotyping, Neuroblastoma, hematogones, hemic and lymphatic diseases, Diseases::Neoplasms::Neoplasms by Histologic Type::Leukemia::Leukemia, Lymphoid::Precursor Cell Lymphoblastic Leukemia-Lymphoma [Medical Subject Headings], medicine, Leucemia, Anatomy::Cells::Blood Cells::Leukocytes::Leukocytes, Mononuclear::Lymphocytes::B-Lymphocytes::Precursor Cells, B-Lymphoid [Medical Subject Headings], cytomegalovirus, Hepatitis, Leukemia, business.industry, infants, leukemia, Lactante, Organisms::Viruses::DNA Viruses::Herpesviridae::Betaherpesvirinae::Cytomegalovirus [Medical Subject Headings], lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, medicine.disease, Pancytopenia, Thrombocytopenic purpura, Leucemia-Linfoma Linfoblástico de Células Precursoras, Células Precursoras de Linfocitos B, medicine.anatomical_structure, Oncology, Citomegalovirus, Bone marrow, Named Groups::Persons::Age Groups::Infant [Medical Subject Headings], business, Infants

Abstract

Hematogones are normal B-lymphoid precursors that multiply in the bone marrow of small children and of adults with ferropenic anaemia, neuroblastoma or idiopathic thrombocytopenic purpura. They are not normally found in peripheral blood, and the immunophenotype is virtually indistinguishable from that of B lymphoblasts. We discuss the case of a 3-month infant with an active cytomegalovirus infection, with hepatitis and pancytopenia associated with 13% hematogones in the bone marrow.

Published

2008

41. Physical and functional characterization of the genetic locus of IBtk, an inhibitor of Bruton's tyrosine kinase: Evidence for three protein isoforms of IBtk

Author

Rosanna Capparelli, Carmen Spatuzza, Marco Schiavone, Notis Argiriou, Marco Sardiello, Giuseppe Scala, Giuseppe Fiume, Olga Fierro, Marco Simonetta, Emanuela Di Salle, Raffaella Faraonio, I. Quinto, Elzbieta Janda, Spatuzza, C., Schiavone, M., Di Salle, E., Janda, E., Sardiello, M., Fiume, G., Fierro, O., Simonetta, M., Argiriou, N., Faraonio, Raffaella, Capparelli, Rosanna, Quinto, I., and Scala, G.

Subjects

Gene isoform, Protein Structure, Evolution, RNA Splicing, NF-KAPPA-B, Messenger, X-linked agammaglobulinemia, Gene Regulation, Chromatin and Epigenetics, Cell Line, Animals, Carrier Proteins, Computational Biology, Evolution, Molecular, Humans, Intracellular Signaling Peptides and Proteins, Promoter Regions, Genetic, Protein Isoforms, Protein Structure, Tertiary, RNA, Messenger, Promoter Regions, Genetic, hemic and lymphatic diseases, PLECKSTRIN HOMOLOGY DOMAINS, medicine, Genetics, Bruton's tyrosine kinase, Kinase activity, Gene, Adaptor Proteins, Signal Transducing, PRE-B CELLS, biology, X-LINKED AGAMMAGLOBULINEMIA, Intron, Molecular, medicine.disease, RNA splicing, biology.protein, RNA, TRANSCRIPTIONAL ACTIVITY, Tyrosine kinase, Tertiary

Abstract

Bruton's tyrosine kinase (Btk) is required for B-cell development. Btk deficiency causes X-linked agammaglobulinemia (XLA) in humans and X-linked immunodeficiency (Xid) in mice. Btk lacks a negative regulatory domain and may rely on cytoplasmic proteins to regulate its activity. Consistently, we identified an inhibitor of Btk, IBtk, which binds to the PH domain of Btk and down-regulates the Btk kinase activity. IBtk is an evolutionary conserved protein encoded by a single genomic sequence at 6q14.1 cytogenetic location, a region of recurrent chromosomal aberrations in lymphoproliferative disorders; however, the physical and functional organization of IBTK is unknown. Here, we report that the human IBTK locus includes three distinct mRNAs arising from complete intron splicing, an additional polyadenylation signal and a second transcription start site that utilizes a specific ATG for protein translation. By northern blot, 5'RACE and 3'RACE we identified three IBTKalpha, IBTKbeta and IBTKgamma mRNAs, whose transcription is driven by two distinct promoter regions; the corresponding IBtk proteins were detected in human cells and mouse tissues by specific antibodies. These results provide the first characterization of the human IBTK locus and may assist in understanding the in vivo function of IBtk.

Published

2008

42. Defining cell-surface antigenic markers for mouse T and B cells.

Author

Raff, Martin C.

Subjects

ISOANTIGENS, LYMPHOCYTES, LABORATORY mice, THYMUS, IMMUNE serums, CELL transformation, T cells

Abstract

The author focuses on the articles by Martin C. Raff regarding the isoantigen and peripheral lymphocytes in mice. Topics discussed include the death of thymus lymphocytes due to antiserum, the analysis of the cells involved an adoptive cell-transfer system for the evaluation of the spleen cells, and the prolonged and frustrating search for T cells.

Published

2014

43. Transplanted long-term cultured pre-BI cells expressing calpastatin are resistant to B cell receptor–induced apoptosis

Author

Ruíz Vela, Antonio, Serrano Gómez, Fernando, González de la Peña, Manuel Ángel, Abad, José Luis, Bernad, Antonio, Maki, Masatoshi, and Martínez-Alonso, Carlos

Subjects

ComputingMilieux_GENERAL, Calpain, pre-B cells, ComputingMilieux_LEGALASPECTSOFCOMPUTING, Transplant, BCR, Calpastatin

Abstract

Copyright © by The Rockefeller University Press, Long-term cultured pre-B cells are able to differentiate into immunoglobulin (Ig)M-positive B cells (IgM cells) when transplanted into severe combined immunodeficient (SCID) mice. Based on previous studies, here we report the development of a reconstitution assay in nonobese diabetic/SCID (NOD/SCID) mice using pre-B cells, which allows us to study the role of calpains (calcium-activated endopeptidases) during B cell development as well as in B cell clonal deletion. Using this model, we show that calpastatin (the natural inhibitor of calpains) inhibits B cell receptor–induced apoptosis in IgM cells derived from transplanted mice. We thus hypothesize an important function for calpain in sculpting the B cell repertoire.

Published

2001

44. Construction of an antigenic map for human B-cell precursors

Author

Melink, Georgiann B. and LeBien, Tucker W.

Published

1983

45. Immunoglobulin isotype expression of normal pre-B cells as determined by immunofluorescence

Author

Kubagawa, Hiromi, Gathings, William E., Levitt, Daniel, Kearney, John F., and Cooper, Max D.

Published

1982

46. Pre-B cells in agammaglobulinemia: Evidence for disease heterogeneity among affected boys

Author

Landreth, Kenneth S., Engelhard, Dan, Anasetti, Claudio, Kapoor, Neena, Kincade, Paul W., and Good, Robert A.

Published

1985

47. Pre-B cells: Normal and abnormal development

Author

Cooper, Max D.

Published

1981

48. Human pre-B cell receptor signal transduction: evidence for distinct roles of PI3kinase and MAP-kinase signalling pathways.

Author

Anbazhagan K, Rabbind Singh A, Isabelle P, Stella I, Céline AD, Bissac E, Bertrand B, Rémy N, Naomi T, Vincent F, Rochette J, and Lassoued K

Abstract

Pre-BCR acts as a critical checkpoint in B cell development. However, its signalling cascade still remains indistinctly characterised in human. We investigated pre-BCR signalling pathway to examine its regulation in normal primary pre-B lymphocytes and pre-B cell lines. In cell lines, early signalling events occurring after pre-BCR stimulation include phosphorylation of Lyn, Blk and Syk together with ZAP70, Btk, Vav, PLC-γ2 and various adaptor proteins, such as BLNK, LAB, LAT and SLP-76. Further downstream, these molecules induced activation of the PI3K/AKT and MAP-kinase resulting in an augmentation of canonical NF-κB pathways and cFos/AP1 activation. PI3K and MAPK exerted opposing effects on the pre-BCR-induced activation of the canonical NF-κB and c-Fos/AP1 pathways. Immediate nuclear export of FoxO3A and delayed import of IRF4 were additional events observed after pre-BCR crosslinking in primary cells. Pre-BCR-induced down-regulation of Rag1, Rag2, E2A and Pax5 transcripts occurred in a PI3K-dependent manner. Finally we bring evidence that pre-BCR stimulation or co stimulation with CD19 enhances cell cycle signal.

Published

2013

49. The presence of precursors of benign pre-B lymphoblasts (hematogones) in the bone marrow of a paediatric patient with cytomegalovirus infection.

Author

Moreno-Madrid F, Uberos J, Díaz-Molina M, Ramírez-Arredondo A, Jiménez-Gámiz P, and Molina-Carballo A

Abstract

Hematogones are normal B-lymphoid precursors that multiply in the bone marrow of small children and of adults with ferropenic anaemia, neuroblastoma or idiopathic thrombocytopenic purpura. They are not normally found in peripheral blood, and the immunophenotype is virtually indistinguishable from that of B lymphoblasts. We discuss the case of a 3-month infant with an active cytomegalovirus infection, with hepatitis and pancytopenia associated with 13% hematogones in the bone marrow.

Published

2008

50. Growth of pre-B cells in cultures of bone marrow from children with acute lymphoblastic leukaemia and other diseases

Author

PAOLO PAOLUCCI, Rapson, N. T., Layward, L., and Hayward, A. R.

Subjects

B-Lymphocytes, bone marrow, Adolescent, acute lymphoblastic leukaemia, Cell Survival, Cytochalasin B, pre-B cells, Hematopoietic Stem Cells, Leukemia, Lymphoid, Bromodeoxyuridine, children, Child, Preschool, Humans, Cycloheximide, Child, Colchicine, Cell Division, Cells, Cultured, Research Article

Abstract

Pre-B cells from the bone marrow of children with acute lymphoblastic leukaemia (ALL) survived up to 144 hr after the completion of treatment and divided in culture with maximum cell numbers at 24 hr. There was no rise in B cell number and no evidence of differentiation from pre-B to B cells. Binucleated pre-B cells in cultures containing cytochalasin B confirmed that pre-B cell division was occurring. Cycloheximide reduced cell numbers in culture but bromodeoxyuridine did not. Pre-B cell numbers also increased in culture of morphologically normal marrows from treated and untreated patients with solid tumours, and probably in normal marrows from patients with non-malignant diseases.

Published

1981