Galectin-9 binds IgM-BCR to regulate B cell signaling

The galectin family of secreted lectins have emerged as important regulators of immune cell function; however, their role in B-cell responses is poorly understood. Here we identify IgM-BCR as a ligand for galectin-9. Furthermore, we show enhanced BCR microcluster formation and signaling in galectin-...

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Veröffentlicht in:Nature communications 2018-08, Vol.9 (1), p.3288-18, Article 3288
Hauptverfasser: Cao, Anh, Alluqmani, Nouf, Buhari, Fatima Hifza Mohammed, Wasim, Laabiah, Smith, Logan K., Quaile, Andrew T., Shannon, Michael, Hakim, Zaki, Furmli, Hossai, Owen, Dylan M., Savchenko, Alexei, Treanor, Bebhinn
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Sprache:eng
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Zusammenfassung:The galectin family of secreted lectins have emerged as important regulators of immune cell function; however, their role in B-cell responses is poorly understood. Here we identify IgM-BCR as a ligand for galectin-9. Furthermore, we show enhanced BCR microcluster formation and signaling in galectin-9-deficient B cells. Notably, treatment with exogenous recombinant galectin-9 nearly completely abolishes BCR signaling. We investigated the molecular mechanism for galectin-9-mediated inhibition of BCR signaling using super-resolution imaging and single-particle tracking. We show that galectin-9 merges pre-existing nanoclusters of IgM-BCR, immobilizes IgM-BCR, and relocalizes IgM-BCR together with the inhibitory molecules CD45 and CD22. In resting naive cells, we use dual-color super-resolution imaging to demonstrate that galectin-9 mediates the close association of IgM and CD22, and propose that the loss of this association provides a mechanism for enhanced activation of galectin-9-deficient B cells. The galectin family of secreted lectins are important regulators of immune cell function; however, their role in B cell responses is poorly understood. Here, the authors identify IgM-BCR as a ligand for galectin-9. In resting naive cells, they show that galectin-9 mediates a close association between IgM and CD22.
ISSN:2041-1723
2041-1723
DOI:10.1038/s41467-018-05771-8