TSC2 S1365A mutation potently regulates CD8+ T cell function and differentiation and improves adoptive cellular cancer therapy
Chirag H. Patel, Yi Dong, Navid Koleini, Xiaoxu Wang, Brittany L. Dunkerly-Eyring, Jiayu Wen, Mark J. Ranek, Laura M. Bartle, Daniel B. Henderson, Jason Sagert, David A. Kass, Jonathan D. Powell
Chirag H. Patel, Yi Dong, Navid Koleini, Xiaoxu Wang, Brittany L. Dunkerly-Eyring, Jiayu Wen, Mark J. Ranek, Laura M. Bartle, Daniel B. Henderson, Jason Sagert, David A. Kass, Jonathan D. Powell
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Research Article Cell biology Immunology

TSC2 S1365A mutation potently regulates CD8+ T cell function and differentiation and improves adoptive cellular cancer therapy

Abstract

MTORC1 integrates signaling from the immune microenvironment to regulate T cell activation, differentiation, and function. TSC2 in the tuberous sclerosis complex tightly regulates mTORC1 activation. CD8+ T cells lacking TSC2 have constitutively enhanced mTORC1 activity and generate robust effector T cells; however, sustained mTORC1 activation prevents generation of long-lived memory CD8+ T cells. Here we show that manipulating TSC2 at Ser1365 potently regulated activated but not basal mTORC1 signaling in CD8+ T cells. Unlike nonstimulated TSC2-KO cells, CD8+ T cells expressing a phosphosilencing mutant TSC2-S1365A (TSC2-SA) retained normal basal mTORC1 activity. PKC and T cell receptor (TCR) stimulation induced TSC2 S1365 phosphorylation, and preventing this with the SA mutation markedly increased mTORC1 activation and T cell effector function. Consequently, SA CD8+ T cells displayed greater effector responses while retaining their capacity to become long-lived memory T cells. SA CD8+ T cells also displayed enhanced effector function under hypoxic and acidic conditions. In murine and human solid-tumor models, SA CD8+ T cells used as adoptive cell therapy displayed greater antitumor immunity than WT CD8+ T cells. These findings reveal an upstream mechanism to regulate mTORC1 activity in T cells. The TSC2-SA mutation enhanced both T cell effector function and long-term persistence/memory formation, supporting an approach to engineer better CAR-T cells for treating cancer.

Authors

Chirag H. Patel, Yi Dong, Navid Koleini, Xiaoxu Wang, Brittany L. Dunkerly-Eyring, Jiayu Wen, Mark J. Ranek, Laura M. Bartle, Daniel B. Henderson, Jason Sagert, David A. Kass, Jonathan D. Powell

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Figure 2

Identification of a TSC regulatory node (S1365) in T cells.

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Identification of a TSC regulatory node (S1365) in T cells. (A) TSC2 pro...
(A) TSC2 protein map shows S1365 relative to other known activating (green) and inhibitory (red) phosphorylation sites for the mouse protein. The human protein is highly homologous in this region, but S1365 in mice is S1364 in human. (B) Immunoblot analysis of T cells before and after stimulation with TCR agonist (αCD3) + Co-Stim with αCD28 after 15, 30, or 60 minutes. (C) Similar study as in B but using αCD3 stimulus alone versus PMA or IL-2. (D) T cells were exposed to increasing concentrations (0.01 mM, 0.1 mM, 1 mM) of H2O2 for 30 minutes and assayed by immunoblot analysis as indicated. PMA is a positive control. (E) T cells were stimulated with PMA in the presence of vehicle (Veh), rapamycin, a selective p38 inhibitor (p38i), ERK inhibitor (ERKi), or PKC inhibitor (PKCi). The p38 inhibitor and, to a lesser extent, the PKC inhibitor blocked phosphorylation at TSC2 (S1365). (F) Pulldown experiment using Flag tagged TSC2 protein expressed in TSC2 KO HEK 293T cells and IP: Flag. Immune complexes incubated with ERK (positive control) or increasing concentration of active p38 and 32P-ATP. The 32P autoradiography band shows label incorporation in TSC2 by both ERK and p38. Total TSC2 detected by Ab-TSC2 or FLAG shown below. (G) Effect of gene silencing (g1) of p38α by CRISPR-CAS9 in naive T cells subsequently activated with combined αCD3 and αCD28 and expanded with IL-2. Immunoblots are from CD8+ T cells isolated on day 7 and stimulated with PMA for 30 minutes. White line denotes separation of lanes from the same gel comparing control (Ctrl) and p38 KO (g1) conditions. Data are representative of at least 3 independent experiments (BE), and 2 independent experiments (G).