CD45 ligation expands Tregs by promoting interactions with DCs
Geoffrey Camirand, … , Christopher E. Rudd, David M. Rothstein
Geoffrey Camirand, … , Christopher E. Rudd, David M. Rothstein
Published September 9, 2014
Citation Information: J Clin Invest. 2014;124(10):4603-4613. https://doi.org/10.1172/JCI74087.
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CD45 ligation expands Tregs by promoting interactions with DCs

Abstract

Regulatory T cells (Tregs), which express CD4 and FOXP3, are critical for modulating the immune response and promoting immune tolerance. Consequently, methods to expand Tregs for therapeutic use are of great interest. While transfer of Tregs after massive ex vivo expansion can be achieved, in vivo expansion of Tregs would be more practical. Here, we demonstrate that targeting the CD45 tyrosine phosphatase with a tolerogenic anti-CD45RB mAb acutely increases Treg numbers in WT mice, even in absence of exogenous antigen. Treg expansion occurred through substantial augmentation of homeostatic proliferation in the preexisting Treg population. Moreover, anti-CD45RB specifically increased Treg proliferation in response to cognate antigen. Compared with conventional T cells, Tregs differentially regulate their conjugation with DCs. Therefore, we determined whether CD45 ligation could alter interactions between Tregs and DCs. Live imaging showed that CD45 ligation specifically reduced Treg motility in an integrin-dependent manner, resulting in enhanced interactions between Tregs and DCs in vivo. Increased conjugate formation, in turn, augmented nuclear translocation of nuclear factor of activated T cells (NFAT) and Treg proliferation. Together, these results demonstrate that Treg peripheral homeostasis can be specifically modulated in vivo to promote Treg expansion and tolerance by increasing conjugation between Tregs and DCs.

Authors

Geoffrey Camirand, Ying Wang, Yuning Lu, Yisong Y. Wan, Yan Lin, Songyan Deng, Galip Guz, David L. Perkins, Patricia W. Finn, Donna L. Farber, Richard A. Flavell, Warren D. Shlomchik, Fadi G. Lakkis, Christopher E. Rudd, David M. Rothstein

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Figure 3

Anti-CD45RB does not induce iTregs in adoptively transferred Tconvs.

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Anti-CD45RB does not induce iTregs in adoptively transferred Tconvs. (A)...
(A) Representative flow cytometry plots showing sort gates used to isolate FOXP3+ or FOXP3 CD4+ cells from Foxp3-RFP congenic (Thy1.1) mice (top row) and purity assessment after sort (bottom row). Numbers represent percentage of events in each gate. (B) Representative flow cytometry plots of live CD4+ cells recovered after adoptive transfer of highly purified FOXP3CD4+Thy1.1+ cells (obtained as in A) into WT congenic mice that were then treated with control IgG or anti-CD45RB (examined in spleens on day 10). Numbers indicate average (± SD) percentage of transferred (Thy1.1+CD4+) cells recovered among total live CD4+B220 cells and FOXP3 expression within the Thy1.1+-transferred cell population. (C) Number of FOXP3CD4+ and FOXP3+CD4+ cells from from right column in B after anti-CD45RB, relative to control IgG (n = 9 mice per group from 3 independent experiments).