Most Ig receptors exist as multi-subunit complexes with a unique ligand binding alpha chain and a common signaling FcR gamma-chain. The myeloid Fc gamma RIIa (CD32) appears unique among FcR because both ligand- binding and signaling capacity are found in the alpha chain. Within the cytoplasmic tails of Fc gamma RIIa and FcR gamma-chain similar, but not identical, activatory motifs (ITAMs) have been defined, in which tyrosines play an important role. Previously, Fc gamma RIIa-ITAM was shown to be critical for both proximal and distal activatory functions in IIA1.6 B-cell transfectants. Triggering of interleukin-2 (IL-2) release and antigen presentation was absent in Fc gamma RIIa, but not in FcR gamma-chain receptor complexes. We now assessed the capacity of Fc gamma RIIa wild-type and Fc gamma RIIa/gamma chimeric molecules to trigger IL-2 production and antigen presentation by B cells. Both of these functions could solely be triggered by receptors containing the FcRIIa was capable of functional interaction with FcR gamma-chain, thus reconstituting the capacity to trigger IL-2 release and antigen presentation. These data document qualitative differences between Fc receptor ITAMs.
ARTICLES|
November 1, 1995
Functional differences between two Fc receptor ITAM signaling motifs
IE Van den Herik-Oudijk,
IE Van den Herik-Oudijk
Department of Immunology, University Hospital, Utrecht, The Netherlands.
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MW Ter Bekke,
MW Ter Bekke
Department of Immunology, University Hospital, Utrecht, The Netherlands.
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MJ Tempelman,
MJ Tempelman
Department of Immunology, University Hospital, Utrecht, The Netherlands.
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PJ Capel,
PJ Capel
Department of Immunology, University Hospital, Utrecht, The Netherlands.
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JG Van de Winkel
JG Van de Winkel
Department of Immunology, University Hospital, Utrecht, The Netherlands.
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Blood (1995) 86 (9): 3302–3307.
Citation
IE Van den Herik-Oudijk, MW Ter Bekke, MJ Tempelman, PJ Capel, JG Van de Winkel; Functional differences between two Fc receptor ITAM signaling motifs. Blood 1995; 86 (9): 3302–3307. doi: https://doi.org/10.1182/blood.V86.9.3302.bloodjournal8693302
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