Akt and SHP-1 are DC-intrinsic checkpoints for tumor immunity
Yaron Carmi, … , Michael N. Alonso, Edgar G. Engleman
Yaron Carmi, … , Michael N. Alonso, Edgar G. Engleman
Published November 3, 2016
Citation Information: JCI Insight. 2016;1(18):e89020. https://doi.org/10.1172/jci.insight.89020.
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Research Article Immunology Oncology

Akt and SHP-1 are DC-intrinsic checkpoints for tumor immunity

Abstract

BM-derived DC (BMDC) are powerful antigen-presenting cells. When loaded with immune complexes (IC), consisting of tumor antigens bound to antitumor antibody, BMDC induce powerful antitumor immunity in mice. However, attempts to employ this strategy clinically with either tumor-associated DC (TADC) or monocyte-derived DC (MoDC) have been disappointing. To investigate the basis for this phenomenon, we compared the response of BMDC, TADC, and MoDC to tumor IgG-IC. Our findings revealed, in both mice and humans, that upon exposure to IgG-IC, BMDC internalized the IC, increased costimulatory molecule expression, and stimulated autologous T cells. In contrast, TADC and, surprisingly, MoDC remained inert upon contact with IC due to dysfunctional signaling following engagement of Fcγ receptors. Such dysfunction is associated with elevated levels of the Src homology region 2 domain–containing phosphatase-1 (SHP-1) and phosphatases regulating Akt activation. Indeed, concomitant inhibition of both SHP-1 and phosphatases that regulate Akt activation conferred upon TADC and MoDC the capacity to take up and process IC and induce antitumor immunity in vivo. This work identifies the molecular checkpoints that govern activation of MoDC and TADC and their capacity to elicit T cell immunity.

Authors

Yaron Carmi, Tyler R. Prestwood, Matthew H. Spitzer, Ian L. Linde, Jonathan Chabon, Nathan E. Reticker-Flynn, Nupur Bhattacharya, Hong Zhang, Xiangyue Zhang, Pamela A. Basto, Bryan M. Burt, Michael N. Alonso, Edgar G. Engleman

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Figure 6

Simultaneous SHP-1 and PTEN blockade enables activation of TADC and MoDC.

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Simultaneous SHP-1 and PTEN blockade enables activation of TADC and MoDC...
Gene expression in blood and BM monocytes from the ImmGen data sets analyzed by (A) principal component analysis, hierarchal clustering of (B) genome-wide data and (C) genes in the PI3K/Akt pathway, and (D) the most significantly altered genes closely involved in regulating Akt phosphorylation. Adjusted P values and statistical significance were determined using the Holm-Sidak method with α = 0.05. (E) Western blots of phosphorylated SHIP-1 and nonphosphorylated PTEN in BM monocyte-derived DC (BMDC), blood monocyte-derived DC (MoDC), and tumor-associated DC (TADC). (F) Phosphorylated Akt levels in DC incubated with C57BL/6 alloIgG-LMP tumor cell IC (alloIgG-IC) over levels in tumor cell–stimulated DC in the presence of SHP-1/2 and PTEN inhibitors. Dot plots show arcsinh ratios of pAkt in DC incubated for 10 minutes with alloIgG-IC over baseline levels obtained from tumor cell–stimulated DC. Part of these data also appear in Figure 5C and are here as a reference for comparison. Statistical significance for BMDC was assessed using Student’s t test with Welch’s correction. Statistical significance for MoDC and TADC was determined by 2-way ANOVA with Tukey’s multiple comparisons test. (G) Flow cytometric analysis of MHC II and CD86 expression on DC subsets following overnight incubation with 129/Sv allogeneic IgG-B16 tumor cell immune complexes (alloIgG-IC) and with or without specific phosphatase inhibitors. Graphs show the percentages of DC expressing both MHC II and CD86. Statistical significance was determined by 2-way ANOVA with Sidak’s multiple comparisons test. (H) The rates of tumor recurrence in tumor-resected mice injected with MoDC or TADC preactivated with 129/Sv allogeneic IgG-B16 tumor cell immune complexes (alloIgG-IC) and with or without phosphatase inhibitors. Statistical significance was determined by the log-rank Mantel-Cox test using Bonferroni-adjusted P values. (I) Confocal and (J) flow cytometric analysis of uptake by MoDC from FcγRIIb–/– mice after overnight incubation with CFSE-labeled B16 tumor cells in immune complexes with allogeneic 129/Sv IgG (alloIgG-IC) and with or without PTEN inhibitor. Original magnification, ×40. *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001.