Monoclonal antibodies against leucoagglutinin‐reactive human T lymphocyte surface components: Two antibodies which inhibit cell‐mediated cytotoxicity at a post‐binding stage

Vargas‐Cortes, Mauricio; Hammarström, Marie‐Louise; Hammarström, Sten; Hellström, U.; Perlmann, Peter

doi:10.1002/eji.1830160713

Cited by 3 publications

(2 citation statements)

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“…The two inhibitory MoAb K3G and 3-19-2 showed similar functional properties [31] but differed in their binding characteristics. Thus, 3-19-2 reacted with a very low number of ceils (<0.3-4%), showing an intense immunofluores-cence stain among resting PBL.…”

Section: Discussionmentioning

confidence: 98%

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Monoclonal Antibodies against Leucoagglutinin‐Reactive Human T‐Lymphocyte Surface Components

Berzins¹,

Vargas‐Cortes²,

Ml³

et al. 1988

Scand J Immunol

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A monoclonal antibody, K46M (IgM kappa), obtained after immunization with leucoagglutinin (La)-reactive T-cell surface components, stimulated human lymphocytes to proliferate. It induced maximal proliferation at greater than 20 micrograms IgM/ml after 3-4 days of culture. Cells stimulated by K46M produced interleukin 2 (IL-2) and gamma interferon (IFN-gamma) and expressed receptors for IL-2 and transferrin. The majority of the activated cells were phenotypically T cells as defined by monoclonal antibodies against CD3 and CD2, and an increase in the K46M-positive cells was also observed during the activation period. K46M-activated cells display major histocompatibility complex (MHC)-unrestricted cytotoxicity against several cultured target cells. The frequencies of the cytotoxic and of the proliferative precursor cells were determined using a limiting dilution assay. K46M seems to activate a larger fraction of cytotoxic precursor cells against Molt 4 than against K562, but the statistical significance of these observations requires further exploration. Both K46M or La activated 40% of PBL to proliferate, whereas 70% of PBL were induced by OKT3. However, the frequency of K46M-activated cells was 40% only when the lymphocytes were plated at low cell densities, i.e. less than 0.5 cells per well. At higher densities an inhibition of proliferation was seen that resulted in a biphasic response curve, indicating that the activation of PBL by K46M was not a single hit event. This was not found with either La or OKT3. Whether K46M, in contrast to OKT3 and La, activates a subpopulation with suppressor activity remains to be established.

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Section: Discussionmentioning

confidence: 98%

“…K46M. was abie to stimulate human iymphocytes to proliferation (3] and two (K3G and 3-i9-2) inhibited ceii-mediated cytotoxicity at a post-bindiiig stage [31]. The characteristics of the proliferative response induced by K4f)M are described in the accompanying paper [3].…”

Section: Discussionmentioning

confidence: 99%

Monoclonal Antibodies against Leucoagglutinin‐Reactive Human T‐Lymphocyte Surface Components

Berzins¹,

Vargas‐Cortes²,

Ml³

et al. 1988

Scand J Immunol

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Elevated NK-mediated lysis of Raji and Daudi cells carrying fixed iC3b fragments

Ramos

Nilsson

et al. 1989

Cellular Immunology

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Monoclonal Antibodies against Leucoagglutinin‐Reactive Human T‐Lymphocyte Surface Components

et al. 1988

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The binding specificities of three biologically active anti-lymphocyte monoclonal antibodies (MoAb) (K46M, K3G, and 3-19-2) produced against human T-cell surface components reactive with the mitogenic lectin leucoagglutinin from Phaseolus vulgaris (La) were analysed. K46M is a strong T-cell mitogen, while K3G and 3-19-2 inhibited cell-mediated cytotoxicity. Resting peripheral blood lymphocytes (PBL) contained 4-16% K46M+ cells, 8-35% K3G+ cells, and less than 0.3-4% 3-19-2+ cells. After stimulation with T-cell mitogens the proportion of K46M+ and 3-19-2+ cells increased markedly (mean 59 and 30% positive cells, respectively), while the increase in K3G+ cells was less prominent (38%). K46M-reactive structures were expressed on mature T cells and probably also on B cells. K3G reacted with B and T cells while 3-19-2 showed a broader specificity reacting also with erythrocytes. All three MoAb reacted with lipid extracts of resting and activated PBL as well as with purified neutral glycolipids of lymphoid origin. In addition 3-19-2 reacted with lipid extracts of erythrocytes. K46M immuno-precipitated four surface peptides from lectin-stimulated PBL. Their apparent molecular weights were 53,000, 42,000, and 16,000 (doublet). The 53,000 and 42,000 MW peptides were identified as the alpha and beta chains of the T-cell antigen receptor. The identity of the 16,000 MW peptides is presently unknown. K3G and 3-19-2 did not specifically precipitate any lymphocyte surface peptide.

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Monoclonal antibodies against leucoagglutinin‐reactive human T lymphocyte surface components: Two antibodies which inhibit cell‐mediated cytotoxicity at a post‐binding stage

Cited by 3 publications

References 54 publications

Monoclonal Antibodies against Leucoagglutinin‐Reactive Human T‐Lymphocyte Surface Components

Monoclonal Antibodies against Leucoagglutinin‐Reactive Human T‐Lymphocyte Surface Components

Elevated NK-mediated lysis of Raji and Daudi cells carrying fixed iC3b fragments

Monoclonal Antibodies against Leucoagglutinin‐Reactive Human T‐Lymphocyte Surface Components

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