Several lines of evidence support our model. B-cell activation by Ag displayed on a target cell is depressed if the target coexpresses α2,6Sia-containing HKI-272 mw glycoconjugates 14, 25. Furthermore, it has recently been reported that sialylated multivalent Ags engage CD22 in trans and inhibit B-cell activation 15. Since α2,6-sialylation is largely a feature of higher eukaryotes, this interaction of CD22 may serve to dampen the B-cell response to self-Ags. In addition, sIgM has been identified as a potential CD22 ligand in trans in an α2,6Sia-dependent manner 11. Therefore, Ag/sIgM complexes may act as α2,6Sia-multivalent Ags and induce CD22-mediated negative regulation
of BCR signaling in order to prevent B-cell activation. Indeed, sIgM-deficient mice 26 as well as CD22-defficient mice 27 exhibited autoimmunity, suggesting that sIgM prevents autoimmunity. Therefore, sIgM contributes
to not only the clearance of Ags, but also to CD22-mediated suppression of B-cell activation to maintain tolerance. CD22 as a receptor for IgM appears to induce negative regulation of B-cell activation. We demonstrate ITF2357 in vivo that CD22 is activated efficiently by Ag/sIgM and negatively regulates BCR signaling in a glycan ligand-dependent manner. Our data strongly suggest that CD22 serves as a receptor for sIgM in a glycan ligand-dependent manner in trans. Together with sIgM as a natural glycan ligand in trans, CD22 regulates a negative feedback loop for B-cell activation and may contribute to B-cell tolerance. The retrovirus vectors pMx-CD22 and pMx-ST6GalI have been described previously 16, 28. The mouse myeloma lines J558L, and NP-specific BCR-reconstituted J558L, J558Lμm3, and NP-specific BCR-reconstituted mouse B lymphoma line K46μv were described previously 16, 28,
29. To obtain retrovirus, plasmids were transfected with Plat-E cells 30 by a method of calcium phosphate precipitation. Cells were infected with the retrovirus expressing mouse CD22 and/or ST6GalI. Spleen CD23+ B cells from QM mice and CD22−/− QM mice 9, 17 were purified as described previously Aspartate 31. Mice including WT C57BL/6 mice were maintained under specific pathogen-free conditions according to the guidelines set forth by the animal committee of Tokyo Medical and Dental University. Cells were cultured as described previously 18. Cells were stimulated with NP-conjugated BSA, or alternatively NP-conjugated sIgM (NP-sIgM) or sialidase (Roche Applied Science)-treated NP-sIgM. Cell lysates were immunoprecipitated with rabbit anti-mouse CD22 Ab 32, anti-SHP-1 Ab, anti-SHIP-1 (these two Abs were from Santa Cruz Biotechnology), anti-FcγRII/III mAb 2.4G2 (BD Biosciences) or NP-specific IgG Ab from QM mice together with protein G-Sepharose (Amersham Pharmacia Biotech). Total cell lysates or immunoprecipitates were separated on SDS-PAGE and transferred to membranes.
No related posts.