5 ± 0.8 ng/mL; mean ± SD; n =9) or granulocyte-rich fraction (fraction 4; 0.9 ± 0.5 ng/mL; mean ± SD; n =9) were around the basal level. There was no additional effect after mixing either of them with the lymphocyte-rich fraction (data not shown). Furthermore, Mac-1+ or Mac-1− plus low+/CD4− cells, but not CD4+ cells, from the macrophage-rich fraction enhanced IgE Ab production when mixed with the lymphocyte-rich fraction. The Mac-1+ cells were phenotypically CD3−/IgM−/B220−/CD11c−/CD14−/Ly-6G−/CCR3− and morphologically mononuclear cells (Fig. 6), suggesting that they were macrophages. These results suggest that cedar pollen might be Romidepsin molecular weight recognized
as an allergen by a mixture of lymphocyte- and macrophage-rich (i.e., Mac-1+ or Mac-1low+) fractions, resulting
in release of IgE Abs from lymphocytes into the culture medium. Next, we incubated various combinations of macrophage- or lymphocyte-rich fraction in submandibular lymph node cells for 6 days and assessed the amounts of IgG Ab in the culture medium (Fig. 7). As expected, bulk submandibular lymph node cells from mice that had been treated i.n. once with the mixture of allergen and adjuvant produced a significant amount of IgG Ab (629.2 ± 92.7 ng/mL; mean ± SD; n= 15). In contrast and unexpectedly, the lymphocyte-rich fraction (fraction 3) of the lymph node cells produced a small amount of IgG Ab (245.7 ± 59.0 ng/mL; mean Napabucasin clinical trial ± SD; n= 15); and the macrophage-rich (fraction 2) fraction was almost inactive (154.2 ± 119.7 ng/mL; Ribonucleotide reductase mean ± SD; n= 15). Of particular interest, IgG Ab production (477.0 ± 135.0ng/mL; mean ± SD; n= 15) was restored by addition of the macrophage-rich fraction (fraction 2) to the lymphocyte-rich fraction (fraction 3). In contrast, the amounts of IgG produced by cells in the damaged cell
(fraction 1; 104.0 ± 24.9 ng/mL; mean ± SD; n= 15)- or granulocyte (fraction 4; 0.0 ± 0.0 ng/mL; mean ± SD; n= 15)-rich fraction were around the basal level; and there was no additional effect after mixing either of them with the lymphocyte-rich fraction (data not shown). Furthermore, Mac-1+ or Mac-1− plus low+/CD4− cells, but not CD4+ cells, from the macrophage-rich fraction enhanced IgG production when mixed with the lymphocyte-rich fraction. These results suggest that cedar pollen injected i.n. with complete Freund’s adjuvant might be recognized as a non-allergenic protein by a mixture of lymphocyte- and macrophage-rich (i.e., Mac-1+ or Mac-1− plus low+/CD4−) fractions, resulting in release of IgG Abs from lymphocytes into the culture medium. To explore which fraction (lymphocyte- or macrophage-rich fraction) is required for class switching of Ig, we injected the allergen alone or with complete Freund’s adjuvant i.n. into BALB/c mice. We then prepared lymphocyte- and macrophage-rich fractions to produce IgE or IgG Abs, respectively; incubated various combinations of these cells for 6 days; and assessed the amounts of IgE or IgG Ab in the culture media (Fig. 8).