The Two Membrane Isoforms of Human IgE Assemble into Functionally Distinct B Cell Antigen Receptors

The human Cε gene expresses two membrane IgE heavy chain mRNAs which differ in the sequence that encodes their extracellular membrane–proximal domain. In the long IgE isoform (m_LIgE), this domain contains a stretch of 52 amino acids which are absent in the short variant (m_SIgE). We have now generated B cell transfectoma cell lines that express these two isoforms and show that both types of mIgE form functional B cell antigen receptors (BCR). Both receptors associate with the Ig-α/Ig-β heterodimer, as well as with protein kinases that are capable of phosphorylating this complex. Upon their cross-linking, both receptors can activate protein tyrosine kinases that phosphorylate the same substrate proteins. Both IgE receptors also associate with two novel proteins that do not bind to mIgM. Apart from these similarities, the two IgE-BCRs show several differences of which some are analogous to the differences between the IgM- and IgD-BCRs. First, the m_SIgE is transported to the cell surface at a higher rate than the m_LIgE. Second, the two IgE-BCRs associate with differently glycosylated Ig-α proteins, the m_LIgE associates with the completely glycosylated form, whereas the m_SIgE associates with an Ig-α glycoform that is partially sensitive to endoglycosidase H. Third, the kinetics of protein tyrosine phosphorylation induced by receptor cross-linking is significantly different for the two IgE-BCRs. Finally, cross-linking of the m_SIgE-BCR leads to growth inhibition of the B cell transfectoma, whereas signaling through the m_LIgE-BCR does not affect the cellular proliferation. These data show that the two human membrane IgE isoforms assemble into functionally distinct antigen receptors which can induce different cellular responses.