TY - JOUR
T1 - Binding of rat IgE with the subcellular components of normal rat mast cells
AU - König, Wolfgang
AU - Ishizaka, Kimishige
N1 - Funding Information:
* This work was supported by research grant AI-10060 from the United States Public Health Service and a grant from the Lillia Babbit Hyde Foundation. This is publication No. 166 from The O'Neill Laboratories of The Good
Funding Information:
Samaritan t Recipient Hospital. of a grant from The Deutsche Forschuugsge-meinschaft Bad Godesberg K~ 427/2.
PY - 1976/4
Y1 - 1976/4
N2 - Attempts were made to obtain subcellular components of rat mast cells which contain receptors for IgE. Rat peritoneal cells were treated with 125I-labeled rat IgE to label mast cells, and disrupted by ultrasonication. More than 90% of cell-bound IgE was recovered in the 20,000 g supernatant fraction which had the ability to block passive cutaneous anaphylaxis with mouse and rat reaginic antibodies. Gel-filtration of the supernatant fraction through a Sepharose 6B column showed that both radioactivity and PCA blocking activity were associated with subcellular components which were eluted in the void volume. When the 20,000 g supernatant fraction of normal peritoneal cells was incubated with 125I-rat IgE, the protein combined with the subcellular components. Incubation of the 20,000 g supernatant with an IgE-rich rat serum inhibited the binding of 125I-IgE with the components, whereas normal rat serum failed to do so. When the sepharose void volume fraction was obtained from purified mast cells and labeled with 125I, approximately 25% of radioactive material was coprecipitated with IgE-anti-IgE complexes. Evidence was obtained that subcellular components of macrophages were not coprecipitated with the antigen-antibody complexes. These results indicated that the components eluted in the void volume fraction contained receptors for IgE. In another experiment, the 20,000 g supernatant fraction was obtained from rat peritoneal cells or purified mast cells whose membrane was labeled with 125I, and fractioned by gel filtration followed by DEAE cellulose chromatography. More than 2 3 of the radioactivity and PCA-blocking activity associated with the sepharose void volume fraction were recovered in the 3 M NaCl fraction which contained 12-15% of total protein. When the 3 M fraction obtained from purified mast cells was labeled with 125I and incubated with an IgE-rich serum, a significant amount of radioactive material in the fraction was precipitated with IgE-anti-IgE complexes. The results indicate that blocking of the PCA reaction by this fraction is due to the presence of receptors for IgE.
AB - Attempts were made to obtain subcellular components of rat mast cells which contain receptors for IgE. Rat peritoneal cells were treated with 125I-labeled rat IgE to label mast cells, and disrupted by ultrasonication. More than 90% of cell-bound IgE was recovered in the 20,000 g supernatant fraction which had the ability to block passive cutaneous anaphylaxis with mouse and rat reaginic antibodies. Gel-filtration of the supernatant fraction through a Sepharose 6B column showed that both radioactivity and PCA blocking activity were associated with subcellular components which were eluted in the void volume. When the 20,000 g supernatant fraction of normal peritoneal cells was incubated with 125I-rat IgE, the protein combined with the subcellular components. Incubation of the 20,000 g supernatant with an IgE-rich rat serum inhibited the binding of 125I-IgE with the components, whereas normal rat serum failed to do so. When the sepharose void volume fraction was obtained from purified mast cells and labeled with 125I, approximately 25% of radioactive material was coprecipitated with IgE-anti-IgE complexes. Evidence was obtained that subcellular components of macrophages were not coprecipitated with the antigen-antibody complexes. These results indicated that the components eluted in the void volume fraction contained receptors for IgE. In another experiment, the 20,000 g supernatant fraction was obtained from rat peritoneal cells or purified mast cells whose membrane was labeled with 125I, and fractioned by gel filtration followed by DEAE cellulose chromatography. More than 2 3 of the radioactivity and PCA-blocking activity associated with the sepharose void volume fraction were recovered in the 3 M NaCl fraction which contained 12-15% of total protein. When the 3 M fraction obtained from purified mast cells was labeled with 125I and incubated with an IgE-rich serum, a significant amount of radioactive material in the fraction was precipitated with IgE-anti-IgE complexes. The results indicate that blocking of the PCA reaction by this fraction is due to the presence of receptors for IgE.
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U2 - 10.1016/0019-2791(76)90346-3
DO - 10.1016/0019-2791(76)90346-3
M3 - Article
C2 - 939578
AN - SCOPUS:0017240092
SN - 0161-5890
VL - 13
SP - 345
EP - 353
JO - Immunochemistry
JF - Immunochemistry
IS - 4
ER -