Glycolytic requirement for NK cell cytotoxicity and cytomegalovirus control
Annelise Y. Mah, Armin Rashidi, Molly P. Keppel, Nermina Saucier, Emily K. Moore, Joshua B. Alinger, Sandeep K. Tripathy, Sandeep K. Agarwal, Emily K. Jeng, Hing C. Wong, Jeffrey S. Miller, Todd A. Fehniger, Emily M. Mace, Anthony R. French, Megan A. Cooper
Annelise Y. Mah, Armin Rashidi, Molly P. Keppel, Nermina Saucier, Emily K. Moore, Joshua B. Alinger, Sandeep K. Tripathy, Sandeep K. Agarwal, Emily K. Jeng, Hing C. Wong, Jeffrey S. Miller, Todd A. Fehniger, Emily M. Mace, Anthony R. French, Megan A. Cooper
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Research Article Immunology

Glycolytic requirement for NK cell cytotoxicity and cytomegalovirus control

Abstract

NK cell activation has been shown to be metabolically regulated in vitro; however, the role of metabolism during in vivo NK cell responses to infection is unknown. We examined the role of glycolysis in NK cell function during murine cytomegalovirus (MCMV) infection and the ability of IL-15 to prime NK cells during CMV infection. The glucose metabolism inhibitor 2-deoxy-ᴅ-glucose (2DG) impaired both mouse and human NK cell cytotoxicity following priming in vitro. Similarly, MCMV-infected mice treated with 2DG had impaired clearance of NK-specific targets in vivo, which was associated with higher viral burden and susceptibility to infection on the C57BL/6 background. IL-15 priming is known to alter NK cell metabolism and metabolic requirements for activation. Treatment with the IL-15 superagonist ALT-803 rescued mice from otherwise lethal infection in an NK-dependent manner. Consistent with this, treatment of a patient with ALT-803 for recurrent CMV reactivation after hematopoietic cell transplant was associated with clearance of viremia. These studies demonstrate that NK cell–mediated control of viral infection requires glucose metabolism and that IL-15 treatment in vivo can reduce this requirement and may be effective as an antiviral therapy.

Authors

Annelise Y. Mah, Armin Rashidi, Molly P. Keppel, Nermina Saucier, Emily K. Moore, Joshua B. Alinger, Sandeep K. Tripathy, Sandeep K. Agarwal, Emily K. Jeng, Hing C. Wong, Jeffrey S. Miller, Todd A. Fehniger, Emily M. Mace, Anthony R. French, Megan A. Cooper

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Figure 4

2DG treatment in vivo confers MCMV susceptibility.

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2DG treatment in vivo confers MCMV susceptibility. Female WT C57BL/6 mic...
Female WT C57BL/6 mice were infected with 1 × 105 PFU murine cytomegalovirus (MCMV) and treated daily with 2-deoxy-ᴅ-glucose (2DG) or PBS. Viral copy number by quantitative PCR from the spleen and liver was measured on (A) day 2 or (B) day 4 after infection, shown as copies of MCMV ie1 gene/copies of β-actin × 1,000 (n = 3–8 individuals/group, 2 experiments, 1-way ANOVA on log-transformed data). (C) Total numbers of lymphocytes and NK cells from the spleen or liver at day 4 after infection. (D) Representative flow cytometry and summary data showing the percentage of BrdU+Ly49H+ NK cells (open) and Ly49H NK cells (hatched), assessed 3 hours after BrdU injection. For C and D, n = 7–8/group, 2 experiments, 1-way ANOVA with Tukey’s multiple comparison test. (E) Survival of uninfected mice compared with infected mice treated with 2DG or PBS (n = 20/group, 4 experiments, log-rank Mantel-Cox test). Data shown as mean ± SEM or survival. *P < 0.05, ***P < 0.001.