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Emergence of a B Lymphocyte Population With ADCC Effector Function in Mammary Tumor Bearing Mice
Author(s) -
Padmanabhan Ranga R.,
Paul Ronald D.,
Watson Gordon A.,
Lopez Diana M.
Publication year - 1988
Publication title -
journal of leukocyte biology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.819
H-Index - 191
eISSN - 1938-3673
pISSN - 0741-5400
DOI - 10.1002/jlb.43.6.509
Subject(s) - antibody dependent cell mediated cytotoxicity , biology , population , cytotoxic t cell , macrophage , splenocyte , immunology , lymphocyte , effector , cytotoxicity , microbiology and biotechnology , antibody , biochemistry , in vitro , medicine , monoclonal antibody , environmental health
Differential expression of antibody dependent cellular cytotoxicity (ADCC) effectors was studied in normal Balb/cCrgl mice and those bearing a chemically induced 7, 12 dimethylbenzanthracene mammary adenocarcinoma. Depletion of macrophages from normal mouse splenocytes by Sephadex G‐10 columns resulted in elimination of ADCC. Further separation of the normal G‐10 nonadherent splenocytes on nylon wool columns did not result in any population with significant cytotoxicity. However, Balb/c mice bearing mammary tumors showed enhanced levels of ADCC which were not eliminated by macrophage removal. Lymphocytes from tumor bearers further separated on nylon wool yielded nonadherent and adherent populations both capable of effecting significant ADCC. Treatment of the nylon nonadherent cells of both normal and tumor bearing mice with anti‐asialo GM 1 (AGM 1 ) and complement decreased the ADCC responses. The same treatment only marginally affected cytotoxic levels of nylon adherent cells from tumor bearers, indicating that these effectors are primarily of non‐NK lineage. In addition, G‐10 nonadherent, nylon adherent cells from tumor bearers separated on a fluorescence activated cell sorter based on the presence of surface immunoglobulins (slg) revealed that both the slg ‐ and slg + (98% pure) sorted cells were capable of functioning in ADCC. To determine whether in the tumor mice the 2% of slg ‐ cells present in the slg + sorted population were the ADCC effectors, mixing experiments were done in which up to 10% of slg ‐ cells from tumor bearers were added to nylon adherent cells from normal mice. No significant increases in ADCC levels were found over that of normal mice. These experiments indicate that the 2% slg ‐ cells were not the ADCC effectors nor were they inducing normal B cells to exert this type of cytotoxic reaction in vitro. To further substantiate the B cell lineage of the slg + ADCC effectors, surface immunoglobulins were removed with protease treatment. After a 36 hr incubation, 92% of the cells had regenerated their slg. The results presented in this paper demonstrate that various splenic lymphoreticular populations from tumor bearers possess an enhanced cytolytic activity against antibody coated target cells. Among these is a unique nylon adherent slg + cell that is capable of functioning as an ADCC effector.