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How J-chain ensures the assembly of immunoglobulin IgM pentamers

Articolo
Data di Pubblicazione:
2025
Citazione:
How J-chain ensures the assembly of immunoglobulin IgM pentamers / Giannone, C.; Mess, X.; He, R.; Chelazzi, M. R.; Mayer, A.; Bakunts, A.; Nguyen, T.; Bushman, Y.; Orsi, A.; Gansen, B.; Degano, M.; Buchner, J.; Sitia, R.. - In: EMBO JOURNAL. - ISSN 0261-4189. - 44:2(2025), pp. 505-533. [10.1038/s44318-024-00317-9]
Abstract:
Polymeric IgM immunoglobulins have high avidity for antigen and complement, and dominate primary antibody responses. They are produced either as assemblies of six µ2L2 subunits (i.e., hexam-ers), or as pentamers of two µ2L2 subunits and an additional protein termed J-chain (JC), which allows transcytosis across epi-thelia. The molecular mechanism of IgM assembly with the desired stoichiometry remained unknown. Here, we show in vitro and in cellula that JC outcompetes the sixth IgM subunit during assembly. Before insertion into IgM, JC exists as an ensemble of largely unstructured, protease-sensitive species with heterogeneous, non-native disulfide bonds. The J-chain interacts with the hydrophobic β-sheets selectively exposed by nascent pentamers. Completion of an amyloid-like core triggers JC folding and drives disulfide rear-rangements that covalently stabilize JC-containing pentamers. In cells, the quality control factor ERp44 surveys IgM assembly and prevents the secretion of aberrant conformers. This mechanism allows the efficient production of high-avidity IgM for systemic or mucosal immunity.
Tipologia CRIS:
1.1 Articolo in rivista
Keywords:
Antibody Biogenesis; ERp44; Mucosal Immunity; Non-Native Disulfides; Protein Quality Control
Elenco autori:
Giannone, C.; Mess, X.; He, R.; Chelazzi, M. R.; Mayer, A.; Bakunts, A.; Nguyen, T.; Bushman, Y.; Orsi, A.; Gansen, B.; Degano, M.; Buchner, J.; Sitia, R.
Autori di Ateneo:
DEGANO MASSIMO
SITIA ROBERTO
Link alla scheda completa:
https://iris.unisr.it/handle/20.500.11768/200488
Pubblicato in:
EMBO JOURNAL
Journal
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