Abstract
Expression of a functional BCR is essential for the development of mature B cells and has been invoked in the control of their maintenance. To test this maintenance function in a new experimental setting, we used the tamoxifen-inducible mb1-CreERT2 mouse strain to delete or truncate either the mb-1 gene encoding the BCR signaling subunit Igα or the VDJ segment of the IgH (H chain [HC]). In this system, Cre-mediated deletion of the mb-1 gene is accompanied by expression of a GFP reporter. We found that, although the Igα-deficient mature B cells survive for >20 d in vivo, the HC-deficient or Igα tail-truncated B cell population is short-lived, with the HC-deficient cells displaying signs of an unfolded protein response. We also show that Igα-deficient B cells still respond to the prosurvival factor BAFF in culture and require BAFF-R signaling for their in vivo maintenance. These results suggest that, under certain conditions, the loss of the BCR can be tolerated by mature B cells for some time, whereas HC-deficient B cells, potentially generated by aberrant somatic mutations in the germinal center, are rapidly eliminated.
Footnotes
This work was supported by research grants provided by the Deutsche Forschungsgemeinschaft through SFB746, TRR130, EXC294, European Research Council Grant 322972 (to M.R.), and European Research Council Grant 268921 (to K.R.) and in part by the Excellence Initiative of the German Research Foundation (GSC-4, Spemann Graduate School) and the Deutsche Forschungsgemeinschaft (SFB 1074 project Z2).
The online version of this article contains supplemental material.
- Received July 29, 2015.
- Accepted December 29, 2015.
- Copyright © 2016 by The American Association of Immunologists, Inc.
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