Differentiation In Vitro of a Leukemia Virus-Induced B-Cell Lymphoma into Macrophages

Mice expressing both a bcl‐2 and a myc transgene within the B lymphoid cell compartment invariably develop novel immature haemopoietic tumours. The likely cell of origin of these tumours was identified by a common pattern of cell surface marker expression on a subset of cells comprising approximately 1% of normal mouse bone marrow. The bcl‐2‐myc tumour cells could be induced to differentiate into either B lymphocytes or macrophages in culture with certain cytokines and feeder cells. Analysis of their progression into the B lymphoid lineage revealed that Igk locus transcription can precede Igh as well as Igk rearrangement. Surprisingly, the undifferentiated tumour cells died rapidly in culture, even in the presence of multiple cytokines, but they proliferated on monolayers of stromal cells derived from haemopoietic tissues. Thus, even with Bcl‐2 levels that protect more differentiated cells, these immature bi‐potential progenitor cells require a stromal‐induced signal for survival. These results provide insight into the process of lineage commitment and suggest new levels of control of cell survival during early steps in haemopoietic development.

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Progenitor tumours from Emu-bcl-2-myc transgenic mice have lymphomyeloid differentiation potential and reveal developmental differences in cell survival.

Strasser

Elefanty

Harris

et al. 1996

The EMBO Journal

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Stage transitions in B-lymphocyte differentiation correlate with limited variations in nuclear proteins.

Rabilloud

Pennetier

Hibner

et al. 1991

Proc. Natl. Acad. Sci. U.S.A.

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Total nuclear proteins extracted from cell lines representing various stages of differentiation of mouse B lymphocytes were studied by computer analysis of twodimensional gels. Of the 1438 spots present on the gels, 55 varied significantly in intensity during differentiation. The variations occurred most often in steps correlating with those classically defined for B-cell differentiation. Seventeen spots were not detectable in at least one of the stages (qualitative variations) and could represent switching on or off of genes coding for nuclear proteins. Detailed analysis of the 55 variable spots showed that they fall into small sets characterized by similar expression profiles, which argues for a combinatorial, multistep control mechanism of gene expression. In addition, analysis of the expression of all the nuclear proteins resolved on the gels clearly differentiated B-lineage cells from myeloid cells and suggested that the most important transition in B-cell differentiation occurs between the resting B cell and plasmocyte stages.Differentiation can be thought of as the acquisition of specialized functions required by complex organisms, which implies that sets of proteins are activated or repressed in each differentiated cell type. As the specific expression of proteins is most often correlated with changes in the gene transcription rate, the question of differentiation can be thought of largely as a problem of transcriptional control. The focus shifts, therefore, to the study of control of gene expression during differentiation. The transcriptional control is generally thought to be mediated by nuclear proteins that bind to regulatory sequences and activate or inactivate transcription. In some model systems (e.g.,-immunoglobulin genes), some of these proteins are known (1). However, little is known about the total extent of the modifications in gene expression upon differentiation and especially on the variations in proteins involved in control of gene expression.We chose to study control of gene expression by a global approach-i.e., the analysis of total nuclear proteins during differentiation. Qualitative or quantitative variations should correlate with subsequent stages of the differentiation process studied and might give information on proteins controlling gene expression. Of the currently available techniques, two-dimensional (2D) gel electrophoresis is best suited for such a global study of protein populations. This approach has been applied to total cell-protein populations mainly for typological studies (2) or to identify polypeptides varying upon transformation (3,4) or during the cell cycle (5). With the recent development of computerized 2D gel processing (for review, see ref. 6) a more complete analysis of the information obtained from 2D gels and the construction of protein data bases is now possible (7). We have, therefore, used computer-analyzed 2D gels to study the variation in nuclear-proteins populations during B-cell differentiation, which is a well-defined multistep process with t...

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Myeloid Antigen, CD13, CD14, and/or CD33 Expression Is Restricted to Certain Lymphoid Neoplasms

et al. 1996

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The authors examined the expression of myeloid antigens (MyAg): CDMb, CDI3, CD14, CD15, and CD33 in 249 adults with lymphoid neoplasms using flow cytometric analysis. In this study, acute leukemia that was myeloperoxidase negative by light microscopy and had at least one lymphoid antigen was defined as acute lymphoblastic leukemia (ALL). The patients were classified as follows: 6 with unclassified ALL, 35 early B precursor ALL, 32 T-ALL, 25 B-cell chronic lymphocytic leukemia (B-CLL) and its variants, 24 B-cell non-Hodgkin's lymphoma (B-NHL), 7 plasma cell disorders, 8 T-CLL, 2 adult T-cell leukemia, and 10 T-NHL. CD1 lb and CD15 were present in a wide range of lymphoid disorders irrespective of B/T lineage and maturity. Unclassified ALL and phenotypically immature ALL frequently expressed CD13Immunophenotypic investigation using comprehensive panels of monoclonal antibodies (MoAbs) to various hematopoietic differentiation antigens have provided unique information for the studies of hematologic neoplasms. 1 ' 2 In a variety of hematologic disorders, investigators have discovered that a substantial proportion of the cases possess characteristics of more than one hematopoietic cell lineage. "6 Among these studies, it is intriguing that many myeloid antigens (MyAgs) can be ex- 10 unlike the range of the expression of lymphoid antigen (LyAg) in acute myelocytic leukemia (AML).6 " However, little is known about the distribution pattern of MyAg expression as to whether it is broadly scattered in lymphoid malignancies or concentrated in certain neoplasms. This issue is fundamentally important to understand the biologic and clinical importance of MyAg in lymphoid neoplasms.In the present study, we investigated the expression of MyAg such as CD1 lb, CD 13, CD 14, CD 15, and CD33 in a whole spectrum of lymphoid malignancies to clarify the distribution characteristics of MyAg expression in relation to the presence of stem cell marker CD34 and chromosomal abnormalities. Our results show that the expression of certain MyAgs such as CD 13, CD 14, and/ or CD33 is relatively restricted to two major groups of lymphoid neoplasms, namely undifferentiated ALL and mature B-cell malignancies. MATERIALS AND METHODS PatientsCell samples were taken from 249 Japanese adult patients (older than 15 years) with lymphoid neoplasms.

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Differentiation In Vitro of a Leukemia Virus-Induced B-Cell Lymphoma into Macrophages

Cited by 9 publications

References 18 publications

Progenitor tumours from Emu-bcl-2-myc transgenic mice have lymphomyeloid differentiation potential and reveal developmental differences in cell survival.

Progenitor tumours from Emu-bcl-2-myc transgenic mice have lymphomyeloid differentiation potential and reveal developmental differences in cell survival.

Stage transitions in B-lymphocyte differentiation correlate with limited variations in nuclear proteins.

Myeloid Antigen, CD13, CD14, and/or CD33 Expression Is Restricted to Certain Lymphoid Neoplasms

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