On the mechanism of internalization of opsonized particles by rat Kupffer cells in vitro

The attachment and internalization of opsonized sheep red blood cells by cultured rat Kupffer cells were studied with phase-contrast and scanning electron microscopy (SEM) as well as timelapse microcinematography. We observed that sheep red cells coated with IgG attached over the entire Kupffer cell surface at random, whereas those coated with IgM and complement attached all over the cell with the exception of the extreme periphery. When the Fc and C₃ receptors were given appropriate stimuli to internalize the attached red cells, they functioned very differently. In Fc internalization, the Kupffer cell membrane rose above the main cell body and wrapped tightly around the attached red cell, eventually surrounding it entirely. In the C₃ internalization, triggered by new-born calf serum, the membrane activity was less spectacular; the folds that did sometimes rise up were coarser and did not fit tightly around the red cell, which was eventually interiorized by a sinking, deep into the cytoplasm of the Kupffer cell. These two mechanisms of internalization also showed different sensitivities to cytochalasin B (CB); the Fc internalization being far more vulnerable to this inhibitor of microfilament activities. Studies with colchicine, however, did not show any clear-cut difference in sensitivity between the two cases.