Cell-targeted PD-1 agonists that mimic PD-L1 are potent T cell inhibitors
Adam P. Curnock, Giovanna Bossi, Jyothi Kumaran, Lindsay J. Bawden, Rita Figueiredo, Rajeevkumar Tawar, Katherine Wiseman, Emma Henderson, Sec Julie Hoong, Veronica Gonzalez, Hemza Ghadbane, David E.O. Knight, Ronan O’Dwyer, David X. Overton, Christina M. Lucato, Nicola M.G. Smith, Carlos R. Reis, Keith Page, Lorraine M. Whaley, Michelle L. McCully, Stephen Hearty, Tara M. Mahon, Peter Weber
Adam P. Curnock, Giovanna Bossi, Jyothi Kumaran, Lindsay J. Bawden, Rita Figueiredo, Rajeevkumar Tawar, Katherine Wiseman, Emma Henderson, Sec Julie Hoong, Veronica Gonzalez, Hemza Ghadbane, David E.O. Knight, Ronan O’Dwyer, David X. Overton, Christina M. Lucato, Nicola M.G. Smith, Carlos R. Reis, Keith Page, Lorraine M. Whaley, Michelle L. McCully, Stephen Hearty, Tara M. Mahon, Peter Weber
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Research Article Immunology

Cell-targeted PD-1 agonists that mimic PD-L1 are potent T cell inhibitors

Abstract

The PD-1/PD-L1 pathway is a key immune checkpoint that regulates T cell activation. There is strong rationale to develop PD-1 agonists as therapeutics against autoimmunity, but progress in this area has been limited. Here, we generated T cell receptor (TCR) targeting, PD-1 agonist bispecifics called ImmTAAI molecules that mimic the ability of PD-L1 to facilitate the colocalization of PD-1 with the TCR complex at the target cell–T cell interface. PD-1 agonist ImmTAAI molecules specifically bound to target cells and were highly effective in activating the PD-1 receptor on interacting T cells to achieve immune suppression. Potent PD-1 antibody ImmTAAI molecules closely mimicked the mechanism of action of endogenously expressed PD-L1 in their localization to the target cell–T cell interface, inhibition of proximal TCR signaling events, and suppression of T cell function. At picomolar concentrations, these bispecifics suppressed cytokine production and inhibited CD8+ T cell–mediated cytotoxicity in vitro. Crucially, in soluble form, the PD-1 ImmTAAI molecules were inactive and, hence, could avoid systemic immunosuppression. This study outlines a promising new route to generate more effective, potent, tissue-targeted PD-1 agonists that can inhibit T cell function locally with the potential to treat autoimmune and chronic inflammatory diseases of high unmet need.

Authors

Adam P. Curnock, Giovanna Bossi, Jyothi Kumaran, Lindsay J. Bawden, Rita Figueiredo, Rajeevkumar Tawar, Katherine Wiseman, Emma Henderson, Sec Julie Hoong, Veronica Gonzalez, Hemza Ghadbane, David E.O. Knight, Ronan O’Dwyer, David X. Overton, Christina M. Lucato, Nicola M.G. Smith, Carlos R. Reis, Keith Page, Lorraine M. Whaley, Michelle L. McCully, Stephen Hearty, Tara M. Mahon, Peter Weber

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Figure 5

H5 ImmTAAI localizes at the target cell–T cell interface and inhibits proximal TCR signaling.

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H5 ImmTAAI localizes at the target cell–T cell interface and inhibits pr...
(A) Schematic of the cell assay used to visualize H5 ImmTAAI localization. (B) Phase contrast and confocal fluorescence images of H5 ImmTAAI localization on ECN90 β cell target cells cocultured with either PD-1+ or PD-1 Jurkat cells. Upper panel: phase contrast. Lower panel: fluorescence images, a white arrow indicates ImmTAAI accumulation (representative images from 3 independent studies). Total original magnification, ×100. (C) The numbers of ECN90 β cell: Jurkat conjugates with ImmTAAI accumulation (white arrow) were counted and plotted as a percentage of the total number of cell conjugates (n = 100 conjugates for conditions using Jurkat Mel5 PD-1 cells and n = 96 for Jurkat Mel5 cells, plotted as mean data from 3 independent studies). (D) Jurkat Mel5 PD-1 cells were stimulated with Melan-A–pulsed ECN90 or ECN90 PD-L1 cells for the indicated times. Whole cell lysates for each condition and time point were resolved by SDS-PAGE, transferred to PVDF membranes, and probed by Western blotting for phospho–SLP-76 (pSLP-76), total SLP-76 (SLP-76), phospho-PLCγ (pPLCγ), total PLCγ (PLCγ), phospho–ZAP-70 (pZAP-70), and total ZAP-70 (representative blots from 3 independent experiments). (E) Jurkat Mel5 PD-1 cells were stimulated with Melan-A–pulsed ECN90 cells, in the presence or absence of H5 ImmTAAI, and Western blots were performed as above (representative blots from 3 independent experiments).