Polymerization of IgA and IgM: Roles of Cys309/Cys414 and the Secretory Tailpiece

Author:

Sørensen Vigdis1,Sundvold Vibeke2,Michaelsen Terje E.3,Sandlie Inger1

Affiliation:

1. *Department of Molecular Cell Biology, Institute of Biology, University of Oslo, Olso, Norway;

2. †Institute of Immunology and Rheumatology, The National Hospital, Oslo, Norway; and

3. ‡Department of Vaccinology, National Institute of Public Health, Oslo, Norway

Abstract

AbstractWe have investigated how the secretory tailpiece (tp), Cys414 and the amino acids flanking Cys414 or Cys309 are involved in regulating the different polymerization of IgM and IgA to pentamers and dimers/monomers, respectively. Whereas changing the tp of IgM to that of IgA has little effect on IgM polymerization, introducing the μtp to IgA leads to the formation of larger than wild-type IgA polymers, including pentamers and hexamer. This shows that the secretory tp can differentially regulate polymerization depending on the heavy chain context. Cys414, which is engaged in intermonomeric disulfide bonds in IgM, is not crucial for the difference in IgM and IgA polymerization; IgM with a C414S mutation forms more large polymers than IgA. Also, IgA with IgM-like mutations in the five amino acids flanking Cys309, which is homologous to Cys414, oligomerize similarly as IgA wild type. Thus, IgA appears to have an inherent tendency to form monomers and dimers that is partially regulated by the tp, while the Cys309 region has only a minor effect. We also show that complement activation by IgM is sensitive to alterations in the polymeric structure, while IgA is inactive in classical complement activation even for polymers such as pentamers and hexamers.

Publisher

The American Association of Immunologists

Subject

Immunology,Immunology and Allergy

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