8 results
Search Results
2. T Cell-dependent Mediator and B-cell Clones.
- Author
-
Lefkovits, I., Quintáns, J., Munro, A., and Waldmann, H.
- Subjects
HEMOCYANIN ,T cells ,SPLEEN ,IMMUNE response ,CELL culture ,ANTIGENS - Abstract
Supernatants were collected from keyhole limpet haemocyanin (KLH) primed spleen cells which had been incubated in tissue culture medium with their priming antigen KLH. These non-specific factor (NSF) containing supernatants were then tested in a microculture system for their ability to facilitate an anti-SRBC response of nu/nu or AT x BM spleen cells. It was concluded that: (a) NSF was able to engage a large number of the available pool of sheep erythrocyte (SRBC) specific B cells into an antibody response; (b) this response was characterized by the development of clones expressing plaque-forming cells (PFC), the number of PFC produced within a clone being dependent upon the amount of NSF available in that culture; (c) NSF probably acted directly on B cells, and not via other accessory cell types. [ABSTRACT FROM AUTHOR]
- Published
- 1975
3. T-cell-derived factor B151-TRF1 IL-5 activates blastoid cells among unprimed B cells to induce a polyclonal differentiation into immunoglobulin M-secreting cells.
- Author
-
Murakami, S., Ono, S., Harada, N., Hara, Y., Katoh, Y., Dobashi, K., Takatsu, K., and Hamaoka, T.
- Subjects
IMMUNOGLOBULINS ,CELL culture ,T cells ,B cells ,CELL differentiation ,ANTIGENS - Abstract
Two distinct murine B-cell differentiation factors, designated B 151 -TRY 1 and B 151-TRF2, were described originally as B151 K12 T-cell hybridoma-derived lymphokines that induce immunoglobulin (Ig) secretion by antigen-activated B cells and unstimulated B cells, respectively. In the present study, we found that a highly purified B1 51-TRF1 fraction prepared by reversed-phase high-performance liquid chromatography (RP-H PLC) also has the ability to cause a polyclonal differentiation of unstimulated B cells into IgM-secreting cells in the apparent absence of co- stimulant. The activity of the B151-TRF1 fraction but not the B151-TRF2 fraction on unstimulated B cells was markedly inhibited by addition of a monoclonal antibody (mAb) specific for the B151- TRF 1/IL-S to the culture. To determine whether 8151 -TRF 1/IL-S and 8151 -TRF2 act on distinct populations among unstimulated B cells, the responsiveness of neonatal B cells and adult B cells that had been fractionated by Percoll density gradient centrifugation was assessed. B15 l-TRFI/IL-5 predominantly acted on lower density B cells, which appeared around 3 weeks after birth in the spleen. In contrast, B151-TRF2 could activate both lower and higher density B cells almost equally and B 151 -TRF2-responsive B cells were already present by 1 week of age. Thus, these results suggest that B151-TRFI/IL-5 and B151-TRF2 act on distinct subpopulations among antigen-unprimed normal B cells to induce IgM-secreting cells. [ABSTRACT FROM AUTHOR]
- Published
- 1988
4. Evaluation of antigen presentation by a murine Ia+ T-cell clone, BK-BI-2.6.C6.
- Author
-
Reske-Kunz, A. B. and Diamantstein, T.
- Subjects
ANTIGENS ,T cells ,LYMPHOCYTES ,IMMUNOGLOBULINS ,CELL culture ,CELL lines ,CYTOKINES ,INTERLEUKINS - Abstract
The capacity of cloned murine Ia-positive BK-BI-2.6.C6 T cells to present protein antigens to antigen-reactive long-term cultured T-cell lines was investigated. Antigen recognition by T-line cells on presenting BK-BI-2.6.C6 T-accessory cells resulted in efficient production of lymphokines. While antigen-dependent T cells with transient interleukin-2 receptor (IL-2R) expression were not induced to proliferate, T cells with constitutive IL-2R expression proliferated in response to the secreted IL-2. Although antigen presentation by BK-BI-2.6.C6 T cells resulted in a slight induction of IL-2R expression on responding T cells, as measured by flow cytometry, this augmentation was much smaller than that induced by antigen-presenting spleen cells. Thus the inability of antigen-presenting T-accessory cells to stimulate proliferation of responding T cells with transient IL-2R expression appears to reflect a lack of signal(s) necessary for the induction of IL-2R up to a level critical for initiation of cell division. This test system represents an ideal model to investigate the nature of signals required, in addition to triggering of the T-cell antigen receptor, for the induction of IL-2R. [ABSTRACT FROM AUTHOR]
- Published
- 1987
5. Mechanism of action of a Db -specific helper clone and factor in cytotoxic responses to alloantigens.
- Author
-
Kwong, P. C. and Teh, H.-S.
- Subjects
T cells ,LYMPHOCYTES ,CELL-mediated cytotoxicity ,ANTIGENS ,IMMUNITY ,CELL culture - Abstract
The mechanism by which a D
b -specific helper clone (clone 9) and a hybridoma-derived Db -especific helper factor, referred to as ASHF, induced cytotoxic T lymphocyte (CTL) responses to alloantigens was investigated. Clone 9 or ASHF helped CBA thymocytes to produce CTL against B6 (H-2b ), but not D2 (H-2d ), alloantigens. However, when BDF1 (H-b,d ) spleen cells or an equal mixture of B6 or D2 spleen cells were used as stimulator cells, CTL responses to both B6 and D2 were induced. This suggested that clone 9 cells or ASHF could induce the production of long-ranged, non-antigen-specific helper factor(s) in B6-stimulated cultures. One of these long-ranged factors produced in B6-stimulated cultures was found to be interleukin-2 (IL-2). Thus, clone 9, which is a non-IL-2 producer, increased the production of IL-2 by irradiated B6 spleen cells and by CBA anti-B6 cultures by 4·7- and 5·7-fold, respectively. ASHF did not increase the amount of IL-2 produced by irradiated B6 spleen cells but increased the amount of IL-2 produced in CBA anti-B6 cultures by 3·8-fold. Clone 9 cells or ASHF did not increase IL-2 production in D2-stimulated cultures. Upon stimulation with concanavalin A or antigen, clone 9 cells also produced a non-antigen-specific helper factor. This factor (IL-X) synergized with excess human recombinant IL.2 (rIL-2) in the polyclonal activation of BDF1 or D2 CTL precursors. A model that involves the participation of ASHF, clone 9 cells, IL-2 and IL-X in the induction of a cytotoxic response is proposed. [ABSTRACT FROM AUTHOR]- Published
- 1987
6. Human cytotoxic T lymphocytes II. FREQUENCY ANALYSIS OF CYCLOSPORIN A-SENSITIVE ALLOREACTIVE CYTOTOXIC T-LYMPHOCYTE PRECURSORS.
- Author
-
Kabelitz, D., Zanker, B., Zanker, C., Heeg, K., and Wagner, H.
- Subjects
CYCLOSPORINE ,T cells ,CELL culture ,ANTIGENS - Abstract
A limiting dilution (LD) culture system was used to investigate the effect of cyclosporin A (CsA) on the activation and differentiation of human alloreactive cytotoxic T-lymphocyte precursors (CTL-p). CsA reduced in a dose-dependent fashion the frequency of alloantigen-inducible CTL-p. With most normal individuals tested there was a 20- to 50-fold reduction of alloreactive CTL-p frequencies in the presence of 500–1000 ng/ml CsA. Both unseparated T cells and CD8
+ T cells were CsA-sensitive under LD culture conditions. Importantly, however, alloreactive CTL-p from two out of 21 normal individuals were found to be largely CsA-resistant. CsA did not affect the growth of MLR-primed CTL in secondary LD culture. Furthermore, CsA slightly inhibited the cytolytic activity of some alloantigen-specific CTL clones. These results arer discussed with respect to the clinical use of CsA in transplantation medicine. [ABSTRACT FROM AUTHOR]- Published
- 1987
7. Autoreactivity developing spontaneously in cultured mouse spleen cells II. COMPARISON OF CYTOTOXICITY OF CULTURED MALE AND FEMALE SPLEEN CELLS.
- Author
-
Gorczynski, R. M.
- Subjects
CELL culture ,FIBROBLASTS ,LYMPHOCYTES ,ANTIGENS ,SPLEEN ,T cells ,LABORATORY mice - Abstract
Male and female spleen cells were compared before and after culture for their cytotoxicity to autologous-embryo fibroblasts. Cultures of male cells developed significantly greater reactivity than cultures of female cells. Moreover, while the cytotoxicity derived from cultures of male cells was totally abolished by treatment of effector cells with a mouse anti-T cells antiserum, such an antiserum had less affect on the effector cells of female mouse cultures. [ABSTRACT FROM AUTHOR]
- Published
- 1976
8. Limiting Dilution Analysis to Helper T-cell Function.
- Author
-
Waldmann, H., Lefkovits, I., and Quintáns, J.
- Subjects
T cells ,DILUTION ,CELL culture ,B cells ,IMMUNE response ,ANTIGENS - Abstract
Limiting dilution analysis has been applied to the study of T-cell 'helper' function in vitro. Using the microculture system one can estimate the numbers of (a) 'helper' T cells involved in specific collaboration with B cells and (b) those T cells which are able, on being activated by their specific antigen, to facilitate the response of B cells to another antigen. Such studies have enabled us to demonstrate that: (1) a single helper' T cell was able to activate a single B-cell precursor to detectable antibody production; (2) the `helper' function of primed T cells was radio-resistant; (3) a minimal estimate of `helper' frequencies could be obtained in defined cell populations; (4) non- specific facilitation was directed towards virtually all available B cells of a given specificity if these were challenged with their appropriate particulate antigen; (5) the microculture system offers the opportunity to determine whether specific and non-specific T-cell helper' effects are a consequence of the activity of one T-cell type or of different subpopulations of T cells. [ABSTRACT FROM AUTHOR]
- Published
- 1975
Discovery Service for Jio Institute Digital Library
For full access to our library's resources, please sign in.