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Start Over Author "Nadler, L. M." Journal journal of immunology baltimore md 1950
32 results on '"Nadler, L. M."'

1. Cloning of BY55, a novel Ig superfamily member expressed on NK cells, CTL, and intestinal intraepithelial lymphocytes.

Author

Anumanthan A, Bensussan A, Boumsell L, Christ AD, Blumberg RS, Voss SD, Patel AT, Robertson MJ, Nadler LM, and Freeman GJ

Subjects
Amino Acid Sequence, Animals, CD28 Antigens blood, CD56 Antigen biosynthesis, CD56 Antigen blood, CD8 Antigens blood, Cloning, Molecular, GPI-Linked Proteins, Glycosylphosphatidylinositols metabolism, Humans, Immunoglobulins chemistry, Intestinal Mucosa cytology, Intestinal Mucosa metabolism, Lymphocyte Activation, Membrane Proteins biosynthesis, Membrane Proteins chemistry, Membrane Proteins immunology, Mice, Molecular Sequence Data, Precipitin Tests, RNA, Messenger biosynthesis, Antigens, CD, Immunoglobulins genetics, Intestinal Mucosa immunology, Killer Cells, Natural metabolism, Lymphocyte Subsets metabolism, Membrane Proteins genetics, Multigene Family immunology, Receptors, Immunologic, T-Lymphocytes, Cytotoxic metabolism
Abstract

Expression of the BY55 protein has been shown to be tightly associated with NK and CD8+ T lymphocytes with cytolytic effector activity. To determine the function of this protein, we molecularly cloned BY55 cDNA. The cDNA sequence predicts a cysteine-rich, glycosylphosphatidylinositol-anchored protein of 181 amino acids with a single Ig-like domain weakly homologous to killer inhibitory receptors. Reduction and carboxyamidomethylation of immunoprecipitated BY55 gave a band of 27 kDa, whereas reduction alone led to an 80-kDa species, suggesting that BY55 is a tightly disulfide-linked multimer. RNA blot analysis revealed BY55 mRNAs of 1.5 and 1.6 kb whose expression was highly restricted to NK and T cells. BY55 was expressed on the CD56dim, CD16+ subset of NK cells, which have high cytolytic activity, but was not expressed and was not induced on the CD56bright, CD16-subset of NK cells, a subset with high proliferative, but low cytolytic, capacity. In human tissues, BY55 mRNA was expressed only in spleen, PBL, and small intestine (in gut lymphocytes). BY55 was expressed on all intestinal intraepithelial lymphocytes, which were predominantly CD3+TCRalpha/beta+CD4-CD8+CD11b+CD28-CD45RO+C D56-CD101+CD103+ (alphaEbeta7 integrin). In addition, BY55 was expressed on most CD8+CD28- peripheral blood T cells. These phenotypic relationships suggest that CD8+CD28+ precursor CTL may terminally differentiate into CD8+CD28-BY55+ effector CTL and that some of the peripheral blood CD8+CD28- subset may represent recirculation from mucosal epithelial immune sites.

Published
1998

2. The BB1 monoclonal antibody recognizes both cell surface CD74 (MHC class II-associated invariant chain) as well as B7-1 (CD80), resolving the question regarding a third CD28/CTLA-4 counterreceptor.

Author

Freeman GJ, Cardoso AA, Boussiotis VA, Anumanthan A, Groves RW, Kupper TS, Clark EA, and Nadler LM

Subjects
3T3 Cells, Abatacept, Amino Acid Sequence, Animals, Antibodies, Blocking pharmacology, Antibodies, Monoclonal pharmacology, Antibody Specificity, Antigens, CD, Antigens, Differentiation immunology, Antigens, Differentiation, B-Lymphocyte genetics, B7-1 Antigen biosynthesis, Binding Sites, Antibody immunology, CD28 Antigens immunology, CHO Cells, COS Cells, CTLA-4 Antigen, Cloning, Molecular, Cricetinae, Histocompatibility Antigens Class II genetics, Humans, Immunoglobulin Fc Fragments metabolism, Interferon-gamma pharmacology, Keratinocytes metabolism, Mice, Molecular Sequence Data, Phenotype, RNA, Messenger biosynthesis, Recombinant Fusion Proteins metabolism, Tumor Cells, Cultured, Antibodies, Monoclonal metabolism, Antigens, Differentiation metabolism, Antigens, Differentiation, B-Lymphocyte immunology, B7-1 Antigen immunology, CD28 Antigens metabolism, Histocompatibility Antigens Class II immunology, Immunoconjugates, Precursor B-Cell Lymphoblastic Leukemia-Lymphoma immunology
Abstract

The identification of all CD28/CTLA-4 counterreceptors is critical to our understanding of this pivotal pathway of T cell activation. Clouding our understanding has been the reported discrepancies in expression and function of the B7-1 (CD80) molecule based upon the use of the BB1 vs other anti-B7-1 mAbs. To resolve this issue, we have cloned a BB1-binding molecule from the BB1+B7-1(-) NALM-6 pre-B cell line. Here, we demonstrate that this BB1-binding molecule is identical to the cell surface form of CD74 (MHC class II-associated invariant chain). CD74-transfected cells bound the BB1 mAb but not other anti-CD80 mAbs, CD28-Ig, or CTLA4Ig. Absorption and blocking experiments confirmed the reactivity of BB1 mAb with CD74. A region of weak homology was identified between CD74 and the region of B7-1 encoding the BB1 epitope. Therefore, the BB1 mAb binds to a protein distinct from B7-1, and this epitope is also present on the B7-1 protein. Many of the puzzling observations in the literature concerning the expression of human B7-1 are resolved by an understanding that BB1 staining is the summation of CD74 plus B7-1 expression. This observation requires the field to reconsider studies using BB1 mAb in the analysis of CD80 expression and function.

Published
1998

3. Induction of T cell clonal anergy results in resistance, whereas CD28-mediated costimulation primes for susceptibility to Fas- and Bax-mediated programmed cell death.

Author

Boussiotis VA, Lee BJ, Freeman GJ, Gribben JG, and Nadler LM

Subjects
3T3 Cells, Animals, Carrier Proteins biosynthesis, Caspase 1, Clone Cells, Cysteine Endopeptidases immunology, DNA Fragmentation immunology, Dimerization, Fas Ligand Protein, Humans, Immunity, Innate, Interleukin-1 antagonists & inhibitors, Interleukin-1 immunology, Ligands, Membrane Glycoproteins biosynthesis, Mice, Proto-Oncogene Proteins chemistry, Proto-Oncogene Proteins c-bcl-2 biosynthesis, Proto-Oncogene Proteins c-bcl-2 chemistry, Proto-Oncogene Proteins c-bcl-2 genetics, Proto-Oncogene Proteins c-bcl-2 immunology, RNA, Messenger biosynthesis, RNA, Messenger immunology, T-Lymphocytes metabolism, Up-Regulation immunology, bcl-2-Associated X Protein, bcl-Associated Death Protein, bcl-X Protein, fas Receptor biosynthesis, Apoptosis immunology, CD28 Antigens physiology, Clonal Anergy, Lymphocyte Activation, Proto-Oncogene Proteins immunology, Proto-Oncogene Proteins physiology, T-Lymphocytes immunology, fas Receptor physiology
Abstract

Since TCR-mediated stimulation induces T cells to become sensitive to Fas-mediated activation-induced cell death (Fas-AICD), we examined whether anergized and CD28-costimulated T cell clones were equally sensitive to Fas-AICD. Here, we show that TCR signal in the presence or absence of CD28 costimulation induced equivalent expression of Fas and Fas ligand. Although anergized cells expressed Fas and Fas ligand, they were resistant to Fas-AICD. Induction of anergy resulted in up-regulation and persistent expression of moderate amounts of bcl-xL and bax and absence of induction of bad. In contrast, CD28-costimulated cells that also expressed Fas and Fas ligand were initially resistant to Fas-AICD but became susceptible after 72 h of culture. Although Fas-mediated apoptosis was the major mechanism of AICD, the IL-1beta-converting enzyme-like protease inhibitor zVAD-FMK totally abrogated DNA fragmentation but not cell death, suggesting that additional Fas-independent apoptotic mechanisms were also operative. Resistance to apoptotic cell death was temporally associated with a dramatic increase of bcl-xL and the presence of bcl-xL:bax heterodimers. Subsequent sensitivity to AICD was associated with down-regulation of bcl-xL, induction of bad, and the displacement of bax from bcl-xL:bax heterodimers. Although induced following CD28 costimulation, bcl-2 did not protect against AICD. Therefore, besides its role in promotion of viability, prevention of anergy, and clonal expansion, CD28 costimulation also has a central role in the induction of subsequent AICD by up-regulating apoptotic mediators.

Published
1997

4. B7-1 is superior to B7-2 costimulation in the induction and maintenance of T cell-mediated antileukemia immunity. Further evidence that B7-1 and B7-2 are functionally distinct.

Author

Matulonis U, Dosiou C, Freeman G, Lamont C, Mauch P, Nadler LM, and Griffin JD

Subjects
Animals, B7-2 Antigen, CD4-Positive T-Lymphocytes immunology, Graft Rejection immunology, Immunotherapy, Adoptive, Mice, Mice, Inbred C3H, Mice, Nude, Neoplasm Transplantation, Tumor Cells, Cultured, Antigens, CD pharmacology, B7-1 Antigen pharmacology, Leukemia, Experimental immunology, Leukemia, Experimental prevention & control, Leukemia, Myeloid immunology, Leukemia, Myeloid prevention & control, Membrane Glycoproteins pharmacology, T-Lymphocytes immunology
Abstract

Although intact, viable tumor cells rarely induce a clinically significant immune response in vivo, immunogenicity can be elicited by irradiated tumor cells that protect against subsequent challenge with wild-type intact viable tumor cells. Genetic modification of murine tumor cells, by transfection of cDNAs encoding either cytokines, MHC molecules, or costimulatory molecules, has been capable of inducing antitumor immunity. We and others have previously demonstrated that expression of the B7-1 costimulatory molecule, in either immunogenic or nonimmunogenic tumors, can protect against subsequent challenge with wild-type tumor cells. In this work, using a murine model of acute myeloid leukemia, we demonstrate that the B7-1 costimulatory molecule is superior to the B7-2 molecule in its capacity to protect against wild-type tumor challenge and eradicate minimal residual disease. These results provide compelling evidence that the B7-1 and B7-2 costimulatory signals are functionally distinct, thus resulting in clinically significant differences in the induction of antitumor immunity in vivo.

Published
1996

5. Differential expression of alternate mB7-2 transcripts.

Author

Borriello F, Oliveros J, Freeman GJ, Nadler LM, and Sharpe AH

Subjects
Amino Acid Sequence, Animals, Antigen-Presenting Cells metabolism, Ascitic Fluid cytology, B-Lymphocytes immunology, B7-2 Antigen, Base Sequence, Mice, Mice, Inbred BALB C, Molecular Sequence Data, Polymerase Chain Reaction, Promoter Regions, Genetic genetics, RNA Processing, Post-Transcriptional genetics, RNA, Messenger analysis, Spleen cytology, Alternative Splicing genetics, Antigens, CD biosynthesis, Antigens, CD genetics, Exons genetics, Membrane Glycoproteins biosynthesis, Membrane Glycoproteins genetics, Transcription, Genetic genetics
Abstract

The murine B7-2 (mB7-2) costimulatory molecule is expressed on APCs early during the course of an immune response, suggesting that it may play a pivotal role in the decision between T cell activation and anergy. Murine B7-2 mRNA displays a restricted pattern of expression; it is inducible in B cells, T cells, NK cells, and dendritic cells, but constitutively expressed in unstimulated monocytes. The constitutive and inducible expression of mB7-2 on distinct cell types indicates that mB7-2 is regulated differentially. To further characterize mB7-2 transcripts, we employed 5' rapid amplification of cDNA ends and reverse transcriptase-PCR to examine transcripts expressed in a variety of types of APCs and analyzed the genomic organization of the mB7-2 gene. We report here that the mB7-2 locus consists of 12 exons and demonstrate that exons 1 through 5 can be used in alternative fashions to produce five distinct transcripts, differing in their 5' untranslated and signal regions. The expression of these transcripts differs in distinct types of APCs and is modulated by stimuli that activate B cells. These results demonstrate that mB7-2 transcripts are differentially regulated in a tissue-specific fashion and in response to activation stimuli.

Published
1995

6. Characterization of the murine B7-1 genomic locus reveals an additional exon encoding an alternative cytoplasmic domain and a chromosomal location of chromosome 16, band B5.

Author

Borriello F, Freeman GJ, Edelhoff S, Disteche CM, Nadler LM, and Sharpe AH

Subjects
Amino Acid Sequence, Animals, B7-1 Antigen chemistry, Base Sequence, Blotting, Northern, Genomic Library, Humans, In Situ Hybridization, Mice, Mice, Inbred AKR, Mice, Inbred DBA, Molecular Sequence Data, Nucleic Acid Hybridization, Polymerase Chain Reaction methods, RNA, Messenger analysis, Alternative Splicing genetics, B7-1 Antigen genetics, Chromosome Mapping, Exons genetics, Transcription, Genetic genetics
Abstract

The murine B7-1 (mB7-1) molecule expressed on APCs delivers a costimulatory signal for T cell activation through its T cell counter-receptor CD28, resulting in T cell proliferation and IL-2 production. Signaling through the TCR in the absence of CD28 signaling results in T cell anergy. We have analyzed the genomic structure of mB7-1 and here describe the identification of a previously unrecognized sixth exon at the far 3' end of the locus, which encodes an alternative cytoplasmic domain. Reverse transcriptase-PCR amplification of mB7-1 transcripts demonstrates that exon 6 is functionally spliced to the transmembrane-encoding exon 4. Furthermore, using 5' rapid amplification of cDNA ends, we determined that the 5'-untranslated region extends over 1505 bp beyond the previously reported transcriptional start site. In addition, we report the chromosomal location of mB7-1 to chromosome 16, band B5.

Published
1994

7. Differential up-regulation of the B7-1 and B7-2 costimulatory molecules after Ig receptor engagement by antigen.

Author

Lenschow DJ, Sperling AI, Cooke MP, Freeman G, Rhee L, Decker DC, Gray G, Nadler LM, Goodnow CC, and Bluestone JA

Subjects
Animals, Antigen-Presenting Cells immunology, Gene Expression, Immune Tolerance, In Vitro Techniques, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Mice, Transgenic, RNA, Messenger genetics, Signal Transduction, T-Lymphocytes immunology, Time Factors, Up-Regulation, B-Lymphocytes immunology, B7-1 Antigen metabolism, Lymphocyte Activation, Receptors, Antigen, B-Cell physiology
Abstract

Ag-pulsed B cells are potent APCs, in part, because of the ability of the Ig receptor to mediate rapid and specific Ag uptake. However, it is also known that full T cell activation requires signals delivered by costimulatory molecules, which naive B cells seem to lack. This study examines the effect Ig receptor engagement has on the expression and function of a new CD28 counter-receptor, B7-2. Unlike B7-1 (B7), B7-2 was rapidly induced on the cell surface of B cells after engagement of the Ig receptor by either anti-Ig mAbs or hen egg lysozyme (HEL) on normal and HEL-specific B cell receptor transgenic B cells, respectively. Furthermore, B7-2 expression was up-regulated on tolerant B cells isolated from HEL/anti-HEL double transgenic mice after Ag stimulation, although at lower levels than on nontolerant transgenic B cells. No significant cell surface levels of B7-1(B7) were observed under these conditions. Finally, the B7-2 molecules induced by Ig cross-linking costimulated T cell proliferation in a CD28-dependent manner, independent of B7-1(B7) expression. Thus, the effectiveness of Ag-specific B cells as APCs depends on both their enhanced Ag uptake, mediated by the B cell receptor, and immediate up-regulation of a potent costimulatory molecule, B7-2.

Published
1994

8. Characterization of CTLA-4 structure and expression on human T cells.

Author

Lindsten T, Lee KP, Harris ES, Petryniak B, Craighead N, Reynolds PJ, Lombard DB, Freeman GJ, Nadler LM, and Gray GS

Subjects
Abatacept, Animals, Antigens, CD analysis, Antigens, Differentiation analysis, Antigens, Differentiation chemistry, Antigens, Differentiation, T-Lymphocyte analysis, Base Sequence, CD28 Antigens, CTLA-4 Antigen, Cell Line, Humans, Immune Sera immunology, Molecular Sequence Data, RNA, Messenger analysis, Rabbits, Antigens, Differentiation genetics, Gene Expression, Immunoconjugates, T-Lymphocytes metabolism
Abstract

CTLA-4 is an adhesion receptor expressed on activated T cells. The amino acid sequence of CTLA-4 is related to CD28, and although the function of CTLA-4 remains unknown, it shares several features with CD28, including a common counter-receptor, B7, that is present on Ag-presenting cells. In a recent study we found that CD28 and CTLA-4 were coexpressed at the mRNA level on activated T cells but that only CD28 was expressed on resting T cells. Here we show that within the T cell population, CTLA-4 expression is restricted to the subset of T cells that also express cell surface CD28. CTLA-4 mRNA expression can be induced on quiescent T cells via phorbol ester-mediated activation of protein kinase C but not with calcium ionophore treatment alone. Phorbol ester-induced expression of CTLA-4 mRNA could be enhanced with calcium ionophore treatment, and treatment of cells in this manner resulted in a reciprocal decrease in expression of CD28 mRNA. Ligation of CD28 with monoclonal antibody also resulted in the specific and rapid induction of CTLA-4 mRNA. To study the expression of CTLA-4 at the protein level, a rabbit antiserum against a recombinant protein derived from CTLA-4 cDNA was generated. When activated T cells were labeled with [35S]methionine, the rabbit antiserum precipitated a 41- to 43-kDa protein from whole cell lysates. Similar results were found when detergent-soluble lysates from 125I surface-labeled resting and activated T cells were analyzed by SDS-PAGE. Surprisingly, under the conditions tested, CTLA-4 migrated primarily as a monomer at the cell surface, and could not be shown to exist as a disulfide-bonded homodimer or as a heterodimer consisting of CTLA-4 and CD28. These results suggest that B7 can bind to T cells via distinct receptor complexes consisting of either CD28 or CTLA-4, and that these complexes may potentially mediate distinct biologic functions. Further, the present results suggest that noncovalent interactions might mediate association of CTLA-4 and/or CD28 at the cell surface.

Published
1993

9. Growth arrest of human B lymphocytes is accompanied by induction of the low molecular weight mammalian heat shock protein (Hsp28).

Author

Spector NL, Samson W, Ryan C, Gribben J, Urba W, Welch WJ, and Nadler LM

Subjects
B-Lymphocytes cytology, Blotting, Western, Heat-Shock Proteins immunology, Hot Temperature, Humans, In Vitro Techniques, Lymphocyte Activation, Phosphorylation, Tetradecanoylphorbol Acetate pharmacology, Time Factors, Tumor Cells, Cultured, B-Lymphocytes physiology, Cell Cycle, Heat-Shock Proteins metabolism
Abstract

A large number of protein and molecular markers have been identified that delineate the early stages of human B cell activation and proliferation. In contrast, few if any molecules are transiently expressed precisely as activated B cells stop proliferating and undergo growth arrest. We demonstrate that the low molecular weight heat shock protein (hsp28) exhibits unique induction kinetics that specifically demarcates this interval. After mitogenic activation of unstimulated splenic B cells, hsp28 protein and phosphorylation transiently increase coinciding precisely with the peak of cellular proliferation and the onset of growth arrest. Although most neoplastic B cells constitutively express hsp28, three cell lines were identified that were hsp28-. No differences in phenotype or growth kinetics were detected between hsp28+ and hsp28- neoplastic B cells demonstrating that hsp28 expression is not essential for cell growth. However, when treated with phorbol ester or heat shock, these hsp28- cell lines synthesize hsp28 followed by the onset growth arrest. The consistency with which hsp28 induction transiently delineates the interval from peak proliferation to the onset of growth arrest suggests hsp28 itself is likely to be involved in regulating this process.

Published
1992

10. Orderly expression of B cell antigens during the in vitro differentiation of nonmalignant human pre-B cells.

Author

Hokland P, Ritz J, Schlossman SF, and Nadler LM

Subjects
Antigens, Differentiation, B-Lymphocyte, Antigens, Neoplasm immunology, B-Lymphocytes cytology, Bone Marrow embryology, Bone Marrow Cells, Cell Differentiation drug effects, Cell Division, Histocompatibility Antigens Class II immunology, Humans, Mitogens, Neprilysin, Receptors, Antigen, B-Cell immunology, Tetradecanoylphorbol Acetate pharmacology, Antigens, Surface immunology, B-Lymphocytes immunology
Abstract

Early human pre-B cells were isolated from fetal bone marrow and induced to differentiate in vitro under the stimulus of phorbol myristic acid or leukocyte-conditioned medium during a 48-hr culture period. Tritiated thymidine culture experiments substantiated that changes in surface marker phenotypes were not the results of outgrowth of subsets responsive to these stimuli. Interestingly, the addition of monoclonal antibodies directed against CALLA resulted in neither proliferation nor differentiation of the fetal lymphoid progenitor cells. Distinct changes in cell surface phenotypes were observed without evidence of cellular enrichment or depletion. The number of CALLA- and TdT-positive cells decreased, whereas the number of B1- and sIgM-positive cells increased. Moreover, a small number of pre-B cells could be driven to a more mature phenotype with the appearance of B2 and sIgG. In contrast, the pan-B B4 antigen did not alter significantly. These changes were even more pronounced when both induction stimuli were present. These studies, and previous studies on the subsets and differentiation of non-T cell acute lymphoblastic leukemias, suggest an orderly acquisition of B cell antigens during the stages of pre-B cell differentiation in man.

Published
1985

11. Structural and functional characterization of IL 2 receptors on activated human B cells.

Author

Boyd AW, Fisher DC, Fox DA, Schlossman SF, and Nadler LM

Subjects
Antibodies, Monoclonal physiology, B-Lymphocytes cytology, B-Lymphocytes immunology, Binding, Competitive, Cell Differentiation, Chemical Phenomena, Chemistry, Physical, Growth Substances physiology, Humans, Interleukin-4, Interphase, Kinetics, Lymphokines physiology, Receptors, Immunologic immunology, Receptors, Immunologic physiology, Receptors, Interleukin-2, Spleen cytology, T-Lymphocytes metabolism, B-Lymphocytes metabolism, Lymphocyte Activation, Receptors, Immunologic analysis
Abstract

After activation, B cells express the IL 2 receptor as determined by their reactivity with monoclonal anti-IL 2 receptor antibodies. In this report we show that anti-IL 2 receptor antibodies precipitated comparable 60,000 to 65,000 dalton proteins from highly purified B and T cells. Limited peptide mapping suggested that the receptors on B and T cells were identical. Moreover, activated B cells could be induced to proliferate by IL 2, but not to secrete Ig. Anti-IL 2R antibody blocked the effect of IL 2 but not the proliferative response induced by B cell growth factor (BCGF), suggesting independent growth factor receptors. Investigation of the kinetics of the B cell response to growth factor indicated that BCGF acts within 24 hr, whereas IL 2 was virtually devoid of activity for 48 hr. Nevertheless, after 72 to 96 hr, the effect of IL 2 was equal to or greater than that obtained with BCGF. These studies suggest that the initial stages of B cell proliferation involves a sequential interaction of BCGF and IL 2 with their respective receptors.

Published
1985

12. Discordant expression of human Ia-like antigens on hematopoietic progenitor cells.

Author

Linch DC, Nadler LM, Luther EA, and Lipton JM

Subjects
B-Lymphocytes immunology, Bone Marrow immunology, Bone Marrow Cells, Colony-Forming Units Assay, HLA-D Antigens, HLA-DP Antigens, HLA-DQ Antigens, HLA-DR Antigens, Hematopoietic Stem Cells cytology, Histocompatibility Antigens Class II genetics, Humans, Monocytes immunology, Polymorphism, Genetic, Hematopoietic Stem Cells immunology, Histocompatibility Antigens Class II immunology
Abstract

The expression of HLA-DR, SB, MT2, and DC antigens on human hematopoietic progenitor cells has been determined by using monoclonal antibodies with complement (C)-mediated cell lysis and immune separation techniques. HLA-DR was detected on greater than 85% of CFU-G/M, myeloid clones (MyCl), BFU-E, and CFU-E. CFU-E were less susceptible to C-mediated lysis at suboptimal C concentrations. The polymorphic MT2 and SB antigens were also present on all categories of progenitor cells, although a lesser proportion of cells were positive. Because in most individuals the antigen density of MT2 and SB, as determined by monoclonal antibody staining, was also lower on B cells and monocytes when compared to HLA-DR expression, the lower number of positive progenitor cells probably reflects lower antigen density rather than distinct positive and negative progenitor cell populations. The DC antigen is expressed weakly on monocytes and B cells, although there is considerable individual variation. In some individuals, distinct DC-positive and -negative monocyte populations are detectable. The DC antigen was not detected on myeloid progenitor cells, even in those individuals with moderate DC expression on their monocytes and B cells. This discordant expression of DC and other Ia-like antigens on hematopoietic progenitor cells may be of physiologic significance and may assist in the purification of progenitor cells from blood and marrow.

Published
1984

13. A monoclonal antibody with reactivity restricted to normal and neoplastic plasma cells.

Author

Anderson KC, Bates MP, Slaughenhoupt B, Schlossman SF, and Nadler LM

Subjects
Animals, Antigen-Antibody Reactions, Antigens, Differentiation, B-Lymphocyte, Antigens, Neoplasm isolation & purification, Antigens, Surface immunology, Cell Line, Cell Transformation, Neoplastic immunology, Female, Humans, Hybridomas immunology, Leukemia, Lymphoid immunology, Leukemia, Plasma Cell immunology, Lymphoid Tissue immunology, Lymphoma immunology, Mice, Mice, Inbred BALB C, Plasma Cells pathology, Plasmacytoma immunology, Antibodies, Monoclonal immunology, Antigens, Neoplasm immunology, Plasma Cells immunology
Abstract

A monoclonal antibody that defines a new and distinct plasma cell antigen, termed PC-1, was developed against human plasmacytoma cells. This antigen is strongly expressed on normal plasma cells isolated from bone marrow and on abnormal plasma cells isolated from myelomas, plasma cell leukemias, and plasmacytomas. The antigen is not detected on normal T or B lymphocytes, granulocytes, or monocytes, and with the exception of plasma cells, is absent on malignancies of B, T, or myeloid origin. Utilizing pokeweed mitogen to induce human B lymphocyte differentiation in vitro, PC-1 is expressed when B cell determinants are lost and the plasmacytoid morphology, intracytoplasmic immunoglobulin-staining, and surface PCA-1- and T10-staining characteristic of plasma cells appear. This antigen is useful for the study of the terminal stages of normal B cell differentiation to plasma cells, and may offer insight into the heterogeneity of the plasma cell dyscrasias.

Published
1984

14. B5, a new B cell-restricted activation antigen.

Author

Freedman AS, Boyd AW, Anderson KC, Fisher DC, Schlossman SF, and Nadler LM

Subjects
Animals, Antibodies, Monoclonal biosynthesis, Antigen-Antibody Reactions, Antigens, Differentiation, B-Lymphocyte, Antigens, Neoplasm analysis, Antigens, Neoplasm immunology, Antigens, Surface isolation & purification, Bone Marrow immunology, Cell Line, Epitopes analysis, Female, Humans, Hybridomas metabolism, Lymphoid Tissue immunology, Mice, Mice, Inbred BALB C, Spleen cytology, Antigens, Surface immunology, B-Lymphocytes immunology, Lymphocyte Activation
Abstract

The characterization of a new human B cell-restricted activation antigen (B5) is described in this report. With the use of a monoclonal antibody to B5, we show that B5 can be detected on peripheral blood or splenic B cells after 1 day of stimulation with either anti-immunoglobulin, protein A, Epstein Barr virus, or pokeweed mitogen. In contrast, B5 was not expressed on resting B, T, or myeloid cells. More important, B5 could not be detected on activated T cells or monocytes. The B5 antigen was expressed on some lymphoblastoid B cell lines and B cell neoplasms but was not expressed on leukemias or lymphomas of T or myeloid origin. The B5 antigen is distinct from previously reported B cell activation antigens by its m.w. and pattern of cellular expression. These studies suggest that B5 is a novel B cell-restricted activation antigen, which may be useful to study the events of early human B cell activation.

Published
1985

15. Characterization of a human B lymphocyte-specific antigen.

Author

Stashenko P, Nadler LM, Hardy R, and Schlossman SF

Subjects
Absorption, Animals, Antibodies, Binding, Competitive, Cell Line, Cytotoxicity, Immunologic, Humans, Hybrid Cells immunology, Leukemia, Experimental immunology, Lymphoma immunology, Mice, Mice, Inbred BALB C, Pokeweed Mitogens pharmacology, B-Lymphocytes immunology, Epitopes
Abstract

A human B lymphocyte-specific antigen (B1) was identified and characterized by the use of a monoclonal antibody. By indirect immunofluorescence, cytotoxicity, and quantitative absorption, B1 was present on approximately 9% of the peripheral blood mononuclear cell fraction and >95% of B cells from blood and lymphoid organs in all individuals tested. Monocytes, resting and activated T cells, null cells, and tumors of T cell and myeloid origin were B1 negative. B1 was distinct from standard B cell phenotypic markers, including Ig and Ia antigen. Removal of the B1 positive population in peripheral blood eliminated all B cells capable or responding to pokeweed mitogen by maturation to Ig-producing cells.

Published
1980

16. Dual fluorochrome analysis of human B lymphocytes: phenotypic examination of resting, anti-immunoglobulin stimulated, and in vivo activated B cells.

Author

Anderson KC, Roach JA, Daley JF, Schlossman SF, and Nadler LM

Subjects
Antibodies, Anti-Idiotypic immunology, Antibodies, Monoclonal, Antigens, Surface analysis, B-Lymphocytes classification, Cell Differentiation, Cells, Cultured, Disease, Flow Cytometry, Humans, Lymphocyte Activation, Lymphoid Tissue cytology, Lymphoid Tissue immunology, Receptors, Immunologic analysis, Receptors, Interleukin-2, Time Factors, B-Lymphocytes immunology
Abstract

B cell-enriched preparations were prepared from human peripheral blood and lymphoid tissues by the depletion of T cells and monocytes. Only B cells by virtue of their staining with anti-B1 conjugated to fluorescein were additionally examined. Dual fluorescence staining and flow cytometric analysis demonstrated that the majority of "resting" human peripheral blood and splenic B cells co-express the B cell-restricted B1 and B2 antigens and lack B5, a B cell-restricted activation antigen, and interleukin 2 receptor (IL 2R). In contrast, nearly 2/3 and 1/3 of B1+ cells isolated from lymph node expressed IL 2R and B5 antigens, respectively. When B1+ B cells from peripheral blood and spleen were "activated" by anti-Ig, they lost the B2 antigen and acquired the B5 and/or IL 2R antigens. 2/3 of B1+ cells strongly expressed IL 2R, and up to 1/2 of B1+ cells co-expressed B5. Delineation of increased numbers of B1+ cells that co-express B5 and/or IL 2R within lymphoid tissues obtained from patients with diseases characterized by "activated" B cells provides in vivo confirmation that these phenotypic changes correlate with B cell activation. We believe that the identification and isolation of these and similar subsets of cells defined by differing cell surface phenotypes should further our understanding both of normal B cell activation and the pathophysiology of B cell disease states.

Published
1986

17. B7, a new member of the Ig superfamily with unique expression on activated and neoplastic B cells.

Author

Freeman GJ, Freedman AS, Segil JM, Lee G, Whitman JF, and Nadler LM

Subjects
Amino Acid Sequence, Antigens, Differentiation, B-Lymphocyte genetics, B-Lymphocytes immunology, Base Sequence, Blotting, Southern, Cell Line, Cloning, Molecular, DNA isolation & purification, Genes, Neoplasm, Hematopoietic Stem Cells analysis, Humans, Molecular Sequence Data, Multigene Family, RNA, Messenger isolation & purification, Sequence Homology, Nucleic Acid, Transfection, Tumor Cells, Cultured immunology, Antigens, Differentiation, B-Lymphocyte isolation & purification, B-Lymphocytes analysis, Lymphocyte Activation, Tumor Cells, Cultured analysis
Abstract

The human B cell restricted activation antigen B7 identifies an in vivo primed subpopulation of B cells that demonstrate an accelerated response to triggers of B cell activation and proliferation. The cDNA encoding B7 was molecularly cloned by cDNA expression. The identity of the B7 cDNA was confirmed by indirect immunofluorescence and immunoprecipitation of a 44/54-kDa protein from B7 transfected COS cells. The sequence of the B7 polypeptide predicts a type I membrane protein of 262 amino acids with eight potential N-linked glycosylation sites in the extracellular region and a short, highly positively charged cytoplasmic tail. The extracellular region is homologous to the Ig gene superfamily and consists of two contiguous Ig-like domains. The first Ig domain has the characteristics of a variable domain and the second that of a constant region domain. B7 mRNA was detected only on anti-Ig activated B lymphocytes and not in other hematopoietic cells. After in vitro activation of B cells with anti-Ig, B7 mRNA was maximally expressed between 4 and 12 h with four RNA transcripts of 1.7, 2.9, 4.2, and 10 kb. The 2.9-kb mRNA predominated in in vitro-activated B cells whereas the 1.7-kb mRNA was most abundant in tumor cells of B cell origin. B7 expression was confined to several histologically defined subgroups of B cell malignancies. The majority of non-Hodgkin's lymphomas were B7+ whereas the B cell leukemias and circulating non-Hodgkin's lymphomas were generally negative. These results demonstrate that the B7 gene encodes a unique molecule belonging to the Ig superfamily and that B7 expression is limited to normal activated B cells and noncirculating B cell malignancies.

Published
1989

18. A monoclonal antibody defining a lymphoma-associated antigen in man.

Author

Nadler LM, Stashenko P, Hardy R, and Schlossman SF

Subjects
Absorption, Animals, Antigens, Surface, Binding, Competitive, Cell Line, Clone Cells immunology, Epitopes, Humans, Hybrid Cells immunology, Leukemia immunology, Lymphocyte Activation, Lymphoid Tissue immunology, Mice, Mice, Inbred BALB C, Receptors, Antigen, B-Cell, Antibodies, Antigens, Neoplasm, Lymphoma immunology
Abstract

A monoclonal antibody (Ab 89) was developed against a lymphoma-associated antigen on the tumor cells of a patient (N.B.) with a B cell, poorly differentiated lymphocytic lymphoma (D-PDL). By indirect immunofluorescence, Ab 89 was shown to react only with N.B. lymphoma cells and was unreactive with normal N.B. lymphoid cells, normal fractionated peripheral blood cells, other normal lymphoid tissues, fetal tissues, and non-lymphoid malignant cells. In addition, Ab 89 was unreactive with conventional immunoglobulins, private and public HLA antigens, or Ia-like antigens. More importantly, Ab 89 was reactive with some B cell lymphoid malignancies. Of the 57 B cell lymphomas tested, it was found that Ab 89 reacted with approximately 10% of B cell D-PDL and B cell chronic lymphocytic leukemia (CLL). Of interest was the finding that N.B. serum contained a circulating antigen which could specifically block the reactivity of Ab 89. The data obtained suggests that Ab 89 defines a tumor-associated antigen shared by a unique subgroup of B cell lymphomas. The group of patients reactive with Ab 89 did not fall into any histopathologic classification system. These data support the notion that there is greater heterogeneity of B cell lymphomas than may have been previously recognized.

Published
1980

19. BLAST-2 [EBVCS], an early cell surface marker of human B cell activation, is superinduced by Epstein Barr virus.

Author

Thorley-Lawson DA, Nadler LM, Bhan AK, and Schooley RT

Subjects
Animals, Antigens, Differentiation, B-Lymphocyte, Antigens, Neoplasm analysis, Antigens, Surface analysis, B-Lymphocytes cytology, Cell Differentiation, DNA biosynthesis, Herpesviridae Infections immunology, Humans, Leukemia immunology, Lymphoma immunology, Tumor Virus Infections immunology, Antigens, Surface isolation & purification, B-Lymphocytes immunology, Cell Transformation, Viral, Herpesvirus 4, Human, Lymphocyte Activation
Abstract

Activation of human B cells by pokeweed mitogen (PWM), protein A, anti-IgM, or EBV infection results in the expression of a new surface antigen, termed BLAST-2 [EBVCS]. This marker appears before the cells undergo blast transformation as assessed by the initiation of DNA synthesis and expression of the BLAST-1 antigen. Thus, the BLAST-2 [EBVCS] antigen is expressed on both activated and lymphoblastoid cells. The antigen is, in addition, restricted to B cells, as it is not found on cells of T or myeloid lineage derived from peripheral blood, cell lines, or neoplastic cells. However, it is readily detected on chronic lymphocytic leukemia cells of B cell origin and in the germinal centers of tonsils and lymph nodes. Like the BLAST-1 antigen, BLAST-2 [EBVCS] is expressed at a high level only on EBV-transformed B lymphoblasts and has a m.w. close to 45,000. Immunoprecipitation experiments show, however, that the two antigens are expressed on distinct populations of molecules.

Published
1985

20. HD39 (B3), a B lineage-restricted antigen whose cell surface expression is limited to resting and activated human B lymphocytes.

Author

Dörken B, Moldenhauer G, Pezzutto A, Schwartz R, Feller A, Kiesel S, and Nadler LM

Subjects
Animals, Antibodies, Monoclonal, Antigens, Differentiation, B-Lymphocyte, Antigens, Neoplasm analysis, Antigens, Surface immunology, B-Lymphocytes cytology, Cell Differentiation, Cell Line, Hematopoietic Stem Cells cytology, Hematopoietic Stem Cells immunology, Leukemia immunology, Lymphoma immunology, Mice, Mice, Inbred BALB C, Antigens, Surface analysis, B-Lymphocytes immunology, Interphase, Lymphocyte Activation
Abstract

The B cell-restricted antigen HD39, whose cell surface expression is limited to resting and activated human B lymphocytes, is described in this report. The monoclonal antibody HD39 detects a two-chain glycoprotein with apparent molecular weights of 130,000 and 140,000. During B cell ontogeny, HD39 is first expressed in the cytoplasm of bone marrow derived pre-B cells, then appears on the cell surface of sIgM+ B cells, and finally on the majority of sIgM+ sIgD+ resting B cells. After activation in vitro, the expression of HD39 on the cell surface first increases, and then the antigen is lost as cells begin to differentiate. HD39 is weakly expressed on very few non-T cell ALL and B cell CLL, on approximately 50% of B cell lymphomas, and not on Waldenström's macroglobulinemias and myelomas. In contrast, it is strongly expressed on all hairy cell leukemias. Its limited cell surface expression in B cell ontogeny suggests that HD39 may be important in the events that regulate the activation of the human resting B lymphocytes.

Published
1986

21. B7, a B-cell-restricted antigen that identifies preactivated B cells.

Author

Freedman AS, Freeman G, Horowitz JC, Daley J, and Nadler LM

Subjects
Animals, Antibodies, Monoclonal immunology, Antigens, Differentiation, B-Lymphocyte immunology, Antigens, Neoplasm analysis, B-Lymphocytes analysis, B-Lymphocytes cytology, Cell Differentiation, Cells, Cultured, Female, Humans, Lymphocyte Activation, Mice, Mice, Inbred BALB C, Spleen cytology, Tumor Cells, Cultured analysis, Antigens, Differentiation, B-Lymphocyte analysis, B-Lymphocytes classification
Abstract

After activation with antigen or mitogen, a number of cell surface proteins appear that are not expressed on resting B cells. To date, a number of B lineage restricted and associated activation antigens have been reported that appear at distinct intervals after in vitro activation. In this report, we describe a new B lineage restricted activation antigen (B7) that appears within 24 hr of in vitro stimulation. The expression of B7 antigen, which is detected on a minor subpopulation of B cells isolated from peripheral blood and lymphoid tissues, is strongly induced following stimulation with either anti-immunoglobulin or Epstein-Barr virus. In contrast, B7 was not detected on resting or activated T cells or monocytes. The B7 antigen was expressed on a subset of B cell lines and B cell neoplasms, but was not detected on leukemias and lymphomas of T cell or myeloid origin. B7 was distinguished from other B cell restricted and associated activation antigens by its unique pattern of expression on a variety of hemopoietic cell lines. The biochemical characterization of B7, that it is a single chain protein of 60 kDa, further distinguishes it from other B cell activation antigens. The functional importance of the B7 antigen was demonstrated when splenic B cells were fractionated into the B7+ and B7- populations. The peak of proliferation in response to anti-Ig, appeared earlier within the B7+ population. These studies suggest that B7 antigen identifies a subpopulation of B cells that are preactivated or primed in vivo, and have an accelerated response to subsequent activation via cross-linking of surface Ig.

Published
1987

22. Antigens on human monocytes identified by monoclonal antibodies.

Author

Todd RF 3rd, Nadler LM, and Schlossman SF

Subjects
Animals, Antigen-Antibody Reactions, Binding Sites, Antibody, Cell Line, Cells, Cultured, Clone Cells immunology, Female, Humans, Leukemia, Lymphoid immunology, Leukemia, Myeloid immunology, Leukocytes immunology, Lymphoma immunology, Mice, Mice, Inbred BALB C, Antibodies, Antigens, Monocytes immunology
Abstract

Two antigens (Mo1 and Mo2) present on human peripheral blood monocytes have been defined by lytic IgM monoclonal antibodies. Both antigens are present on greater than 70% of adherent mononuclear cells (predominantly monocytes). Mo1 is expressed by monocytes, granulocytes, and Null cells, but is absent from T and B lymphocytes. Mo2, on the other hand, appears specific for peripheral blood monocytes. Neither antigen is present on Ia-positive B cell lines or on tumor cells from patients with B cell lymphoproliferative malignancies, further excluding the possibility that Mo1 and Mo2 are Ia antigens. Mo1 and Mo2 are, however, present on a significant number of blast cells from patients with monocytic leukemia (both myelomonocytic and pure monocytic variants), but relatively infrequently expressed by cells from patients with acute granulocytic leukemia. These results indicate that Mo1 and Mo2 are unique antigens that may represent distinct stages of late monocyte-granulocyte differentiation.

Published
1981

23. Pre-exposure of human B cells to recombinant IL-1 enhances subsequent proliferation.

Author

Freedman AS, Freeman G, Whitman J, Segil J, Daley J, and Nadler LM

Subjects
Antibodies, Anti-Idiotypic, B-Lymphocytes immunology, Cells, Cultured, Humans, Interferon-gamma pharmacology, Interleukin-2, Interleukin-4, Interleukins, Palatine Tonsil drug effects, Palatine Tonsil immunology, Spleen drug effects, Spleen immunology, Time Factors, B-Lymphocytes drug effects, Interleukin-1 pharmacology, Lymphocyte Activation drug effects, Recombinant Proteins pharmacology
Abstract

The reported effects of the monocyte-derived cytokine IL-1 on human B lymphocytes are both varied and controversial. IL-1 has been reported to augment both proliferation and Ig secretion of previously activated human B cells. In the present study highly purified splenic B cells were cultured with rIL-1 before, simultaneously with, and after the addition of the polyclonal B cell mitogen, anti-Ig. rIL-1 had no significant effect on B cell proliferation when added simultaneously with or after B cell activation with anti-Ig. However, incubation of splenic B cells with rIL-1 for 24 h before stimulation with anti-Ig appeared to enhance mitogenesis. With the observation that rIL-1 exerted effects on resting B cells, the effect of rIL-1 on several events which accompany B cell activation was examined. rIL-1 failed to stimulate RNA synthesis, effect increases in cell size or intracellular Ca2+ levels, or lead to the hyperexpression of MHC class II or B cell activation Ag. These studies suggest that rIL-1 does not activate B cells but primes them to respond to subsequent activation.

Published
1988

24. Antigens on human plasma cells identified by monoclonal antibodies.

Author

Anderson KC, Park EK, Bates MP, Leonard RC, Hardy R, Schlossman SF, and Nadler LM

Subjects
Animals, Antigens, Differentiation, B-Lymphocyte, B-Lymphocytes immunology, Blood Cells immunology, Female, Humans, Hybrid Cells immunology, Leukemia, Plasma Cell immunology, Lymphocyte Activation, Lymphoid Tissue immunology, Mice, Mice, Inbred BALB C, Multiple Myeloma immunology, Antibodies, Monoclonal immunology, Antigens, Neoplasm analysis, Antigens, Surface analysis, Plasma Cells immunology
Abstract

Two monoclonal antibodies that define distinct plasma cell-associated antigens, termed PCA-1 and PCA-2, were developed against human plasma cell leukemia cells. These antigens are strongly expressed on human myelomas, plasma cell leukemia, and plasmacytoma tumor cells, but are not detected on other lymphoid malignancies of B, T, null, or myeloid origin. PCA-1 and PCA-2 are not expressed on either normal T or B lymphocytes, but are weakly expressed on granulocytes and monocytes. When pokeweed mitogen is used to induce human B lymphocyte differentiation, PCA-1 is expressed when other B cell determinants are lost and plasmacytoid morphology, intracytoplasmic immunoglobulins, and surface T10 staining characteristic of plasma cells appear. In contrast, PCA-2 cannot be induced and may therefore appear later in the B cell differentiation scheme. These antigens may be of utility for the study and regulation of normal and abnormal plasma cell growth, traffic, and tissue distribution and may aid in understanding heterogeneity within plasma cell dyscrasias.

Published
1983

25. Regulatory mechanisms in cell-mediated immune responses. II. Comparison of culture-induced and alloantigen-induced suppressor cells in MLR and CML.

Author

Nadler LM and Hodes RJ

Subjects
Animals, Cell Membrane immunology, Cell Membrane Permeability, Cells, Cultured, Cytotoxicity Tests, Immunologic, In Vitro Techniques, Lymphocyte Culture Test, Mixed, Male, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Mitomycins pharmacology, Spleen cytology, Spleen immunology, Immunity, Cellular, Isoantigens, T-Lymphocytes immunology
Abstract

Two antigen-nonspecific T cell-dependent suppressor systems were compared for their effects upon CML and MLR. Suppressor cells generated by an in vitro culture of spleen cells were compared with suppressor cells generated by in vivo priming with alloantigen. Culture-induced suppressor cells were themselves unable to respond in CML or MLR; were able to suppress actively the CML and MLR responses of untreated responding cells; were mitomycin-sensitive; and, produced no easily demonstrable suppressive supernatant. Alloantigen-primed cells were able to respond in CML and LR; could suppress proliferation in MLR, but were able to suppress CML only after mitomycin treatment; and, produced suppressive supernatants active in suppressing both CML and MLR. In addition to cataloging the differences and similarities between these suppressor populations, the data have been employed to analyze the mechanisms by which suppression occurs in CML and MLR.

Published
1977

26. Isolation and functional analysis of human B cell populations. I. Characterization of the B1+B2+ and B1+B2- subsets.

Author

Anderson KC, Boyd AW, Fisher DC, Slaughenhoupt B, Groopman JE, O'Hara CJ, Daley JF, Schlossman SF, and Nadler LM

Subjects
Acquired Immunodeficiency Syndrome immunology, Acquired Immunodeficiency Syndrome pathology, Antibody-Producing Cells immunology, Antigens, Differentiation, B-Lymphocyte, B-Lymphocytes cytology, B-Lymphocytes immunology, Cell Cycle, Flow Cytometry, Humans, Lymphatic Diseases immunology, Lymphatic Diseases pathology, Lymphocyte Activation, Lymphoid Tissue cytology, Phenotype, Spleen cytology, Antigens, Surface analysis, B-Lymphocytes classification, Cell Separation methods
Abstract

Distinct populations of human B lymphocytes can be identified by their expression and/or co-expression of the B cell-restricted antigens B1 and B2. Dual fluorochrome staining and flow cytometric cell sorting permitted the isolation of the B1+B2+ and B1+B2- cells to homogeneity. In contrast, very few B1-B2+ cells were obtainable from normal lymphoid organs. Virtually all B1+B2+ cells expressed IgM and IgD, but lacked IgG and the plasma cell antigens PCA-1 and PC-1, whereas the B1+B2- cells more frequently expressed IgG, PCA-1 and PC-1. Both populations were noncycling and were composed of similar percentages of small and large cells. The B1+B2+ cells proliferate to anti-mu or to anti-mu + PHA-LCM, but not to PHA-LCM alone. They require both T cells and PWM to produce Ig. In contrast, B1+B2-cells do not significantly proliferate to anti-mu, PHA-LCM, or anti-mu and PHA-LCM. They produce Ig in response to T cells alone without PWM. These phenotypic and functional observations provide preliminary evidence that these populations are distinct and that the B1+B2+ cell may be a "resting" B cell, whereas the B1+B2- cell appears to be more "differentiated." The present studies further suggest that they will also be helpful in characterizing B cells in some human disease states. We believe that the identification and isolation of these and similar subsets of B cells defined by differing cell surface phenotype should aid our understanding both of normal B cell differentiation and of B cell disease states.

Published
1985

27. Ontogeny of human hematopoietic cells: analysis utilizing monoclonal antibodies.

Author

Rosenthal P, Rimm IJ, Umiel T, Griffin JD, Osathanondh R, Schlossman SF, and Nadler LM

Subjects
Antigens, Differentiation, B-Lymphocyte, Antigens, Differentiation, T-Lymphocyte, Antigens, Surface analysis, Bone Marrow immunology, Bone Marrow Cells, Cell Count, Female, Fetus, HLA Antigens analysis, Hematopoietic Stem Cells cytology, Humans, Liver cytology, Lymphoid Tissue, Pregnancy, Receptors, Cell Surface immunology, Receptors, Transferrin, Spleen cytology, beta 2-Microglobulin immunology, Antibodies, Monoclonal immunology, Hematopoiesis, Hematopoietic Stem Cells immunology
Abstract

Lymphoid and myeloid cells isolated from second trimester fetal lymphoid organs were characterized by utilizing a panel of monoclonal antibodies that define human lineage-restricted, differentiation, histocompatibility, and activation antigens. At distinct gestational stages, the appearance of morphologically identifiable lymphoid and myeloid cells paralleled the appearance of cells expressing definable lymphoid and myeloid antigens. The proportion of cells in fetal liver, bone marrow, and spleen that expressed histocompatibility, myeloid, and B cell antigens increased with fetal maturation. In contrast, even the earliest fetal thymuses studied were of a phenotype no different than that seen during later stages of ontogeny. Although the cellular lineage of most fetal hematopoietic cells could be identified by this panel of reagents, a considerable number of fetal liver and bone marrow cells did not express any of these antigens, suggesting the possibility that they might represent early hematopoietic progenitor cells. These studies support the notion that the adult cellular phenotype is the result of both an orderly acquisition of differentiation antigens and the migration of these primitive cellular populations to specific fetal organs. Identification of hematopoietic progenitors in fetal tissues may facilitate the identification and isolation of early lymphoid and myeloid progenitor cells in adults.

Published
1983

28. B4, a human B lymphocyte-associated antigen expressed on normal, mitogen-activated, and malignant B lymphocytes.

Author

Nadler LM, Anderson KC, Marti G, Bates M, Park E, Daley JF, and Schlossman SF

Subjects
Animals, Antigens, Differentiation, B-Lymphocyte, Antigens, Surface immunology, B-Lymphocytes cytology, Cell Differentiation, Cell Line, Female, Flow Cytometry, Fluorescent Antibody Technique, Humans, Leukemia, Lymphoid immunology, Leukemia, Myeloid immunology, Lymphoma immunology, Macrophage-1 Antigen, Mice, Mice, Inbred BALB C, Receptors, Complement analysis, Receptors, Fc analysis, Antigens, Neoplasm analysis, Antigens, Surface analysis, B-Lymphocytes immunology, Lymphocyte Activation
Abstract

The characterization of a new B cell-specific antigen (B4) is described in this report. With the use of a monoclonal antibody to B4, it was shown that B4 is present on B cells isolated from peripheral blood and lymphoid organs, on cell lines derived from normal and malignant B cells, and on tumor cells isolated from patients with B cell-derived neoplasms. B4, in contrast, was not detected on normal, activated, or malignant cells of T or myeloid origin. The B4 antigen is distinct from known B cell antigens, including sIg, Ia, B1, B2, Fc, and C3. Examination of mitogen-stimulated B lymphocytes suggests that the B4 antigen initially increases with B cell activation and then is lost at the terminal stage of B cell differentiation. Moreover, the observation that B4 is expressed on almost all early B cell tumors suggests that it may precede B1, CALLA, cytoplasmic mu, and B2 in early B cell ontogeny.

Published
1983

29. Studies of in vitro activation and differentiation of human B lymphocytes. I. Phenotypic and functional characterization of the B cell population responding to anti-Ig antibody.

Author

Boyd AW, Anderson KC, Freedman AS, Fisher DC, Slaughenhoupt B, Schlossman SF, and Nadler LM

Subjects
Animals, Antigens, Surface analysis, B-Lymphocytes cytology, B-Lymphocytes immunology, Cell Differentiation, Cell Separation methods, Flow Cytometry, Humans, Kinetics, Phenotype, Rabbits, Spleen cytology, Antibodies, Anti-Idiotypic physiology, B-Lymphocytes classification, Lymphocyte Activation
Abstract

Investigation of the activation of splenic B cells by anti-immunoglobulin (Ig) antibody has enabled us to characterize the anti-Ig-responsive B cell and to analyze the phenotypic changes which accompany proliferation and differentiation. The anti-Ig antibody-responsive B cell population was characterized by the expression of high levels of the B2 antigen and represented approximately 40% of splenic B cells. Brisk mitogenesis which peaked at 3 to 4 days was induced by anti-Ig antibody. The proliferative phase was characterized phenotypically by a dramatic decline in B2 antigen expression, with most cells showing no detectable B2 by 4 days post-activation. The other hallmark of this phase was de novo expression of a group of "activation antigens." These included the B cell-restricted antigens B-LAST 1, BB1, and B5, and the T cell-associated interleukin 2 receptor and T12 antigens. Concomitantly, B1, B4, and Ia expression increased, the increase being roughly proportional to the increase in cell size. After day 4, the mitogenic response progressively diminished, while Ig synthesis increased. During this differentiation phase, cell surface antigens again displayed a distinct sequence of changes. The five activation antigens and the B1, B4, and Ia antigens began to decrease. However, two markers, T10 and PCA-1, which are found on plasmacytomas, appeared and their level of expression steadily increased. These changes and the appearance of morphologically identifiable plasma cells required the presence of T cells in this system. T cell supernatants alone induced Ig secretion but did not induce expression of PCA-1 or the appearance of cells with plasma cell morphology. The culture system developed in this study has allowed us to analyze the antigenic changes following activation by anti-Ig antibody. This sequence of changes has not only permitted the identification of antigens which, by their appearance at distinct stages may have an important role in proliferation and differentiation of B cells, but also provides us with the means of studying the function of each antigen.

Published
1985

30. The B cell surface molecule B1 is functionally linked with B cell activation and differentiation.

Author

Tedder TF, Boyd AW, Freedman AS, Nadler LM, and Schlossman SF

Subjects
Adult, Antibodies, Monoclonal physiology, Antigens, Differentiation, B-Lymphocyte, B-Lymphocytes cytology, Binding, Competitive, Growth Substances pharmacology, Humans, Interphase, Microspheres, Time Factors, Antigens, Surface immunology, B-Lymphocytes immunology, Cell Differentiation, Lymphocyte Activation
Abstract

The B1 molecule is a 32,000 m.w. phosphorylated cell surface protein expressed exclusively by B cells from the mid pre-B until the plasma cell stage of differentiation. Two monoclonal antibodies (gamma 2a and mu) reactive with this molecule were used to assess the role of B1 in B cell activation, proliferation, and differentiation. The anti-B1 antibodies at concentrations ranging from 0.1 to 100 micrograms/ml significantly inhibited B cell proliferation induced by anti-mu antibodies, Staphylococcus aureus Cowan strain 1, activated T cells, and Epstein Barr virus. Although capable of inhibiting proliferation, anti-B1 antibody in soluble form or coupled to beads did not activate B cells or induce proliferation. Antibodies of comparable isotypes or against other B cell-restricted antigens, including B2, B4, B5, and HB-5, did not inhibit activation. Pretreatment of B cells with anti-B1 antibody did not inhibit activation, indicating that B cells had to be cultured with anti-B1 antibody for anti-B1-mediated inhibition to occur. Maximum inhibition was obtained when anti-B1 antibody was added at the initiation of culture. In agreement with this, growth factor-dependent proliferation of preactivated B cells was not inhibited by anti-B1 antibodies. Comparable inhibition of B cell activation was noted with antibodies reactive with class II antigens of the major histocompatibility complex with the exception that anti-B1 antibody inhibited immunoglobulin secretion in pokeweed mitogen assays, whereas anti-DR antibody did not. These results suggest that the B1 molecule may serve a central role in the regulation of B cell activation and differentiation.

Published
1985

32. Characterization of a human B cell-specific antigen (B2) distinct from B1.

Author

Nadler LM, Stashenko P, Hardy R, van Agthoven A, Terhorst C, and Schlossman SF

Subjects
Absorption, Animals, Antibodies immunology, Chemical Phenomena, Chemistry, Clone Cells immunology, Female, Fluorescent Antibody Technique, Guinea Pigs, Histocompatibility Antigens Class II immunology, Humans, Lymphoma immunology, Mice, Rabbits, Receptors, Antigen, B-Cell immunology, Receptors, Complement immunology, Receptors, Fc immunology, Antigens classification, B-Lymphocytes immunology, Epitopes
Abstract

A human B lymphocyte-specific antigen (B2) was identified and characterized by the use of a monoclonal antibody. By indirect immunofluorescence and quantitative absorption, B2 was shown to be expressed exclusively on Ig+ B cells isolated from peripheral blood and lymphoid tissues. In contrast, B2 was not found on monocytes, resting and activated T cells, Null cells, or granulocytes, nor was it found on cell lines or tumor cells of T cell or myeloid origin. Functional studies demonstrated that only B2 antigen-positive splenocytes could be induced to differentiate into plasma cells under the stimulus of pokeweed mitogen, further confirming the B cell specificity of B2. It was then demonstrated that the B2 antigen was distinct from the previously described B cell-surface determinants including surface immunoglobulin, Ia-like antigens, and Fc and C3 receptors. More importantly, the B2 antigen has been clearly shown to be distinct from the previously described B cell-specific antigen, B1, by its m.w. and expression on normal and malignant B lymphocytes. The distinct distribution of B2 on normal and malignant lymphocytes supports the notion of B cell heterogeneity and provides further evidence for existence of subpopulations of human B lymphocytes.

Published
1981

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