Abstract
We applied an antibody-dependent macrophage-mediated cytotoxicity (ADMC) test in order to analyze the effector mechanism of the host-mediated antitumor effects induced by OK-432. Adherent peritoneal exudate (PE) cells were obtained from each of high (C3H/He) and low (B10) responder mice treated with OK-432, and 51Cr-labeled MM2 tumor cells were used as target cells. The cytotoxic activity in vitro coincided well with the results obtained in in vivo antitumor experiments. When adherent PE cells from C3H/He mice reacted with anti-MM2 serum from B10 mice, the degree of ADMC was significantly lower than that obtained with the anti-MM2 serum from C3H/He mice. The removal of IgG1 from the anti-MM2 serum induced in B10 mice resulted in the enhancement of ADMC activity. Then mean level of IgG2 in each of anti-MM2 sera from C3H/He and B10 mice was higher than in normal serum, and the IgG1 level in the antiserum from B10 mice was also higher than that in the serum from normal B10 mice. The present work suggested that the active component(s) in anti-MM2 serum participating in ADMC was a specific antibody of the IgG2 subclass, and that the inhibiting factor(s) was the IgG1 subclass.
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