| Literature DB >> 32327756 |
Tobias Baumann1, Andreas Dunkel2, Christian Schmid3, Sabine Schmitt4, Michael Hiltensperger5, Kerstin Lohr1, Vibor Laketa6, Sainitin Donakonda1, Uwe Ahting7, Bettina Lorenz-Depiereux8, Jan E Heil9, Johann Schredelseker10, Luca Simeoni11, Caroline Fecher12, Nina Körber13, Tanja Bauer13, Norbert Hüser14, Daniel Hartmann14, Melanie Laschinger14, Kilian Eyerich15, Stefanie Eyerich16, Martina Anton1, Matthew Streeter17, Tina Wang18, Burkhart Schraven11, David Spiegel17,19, Farhah Assaad20, Thomas Misgeld12, Hans Zischka4,21, Peter J Murray22, Annkristin Heine23,24, Mathias Heikenwälder25, Thomas Korn5, Corinna Dawid3, Thomas Hofmann2,3, Percy A Knolle26,27,28, Bastian Höchst29.
Abstract
Regulatory myeloid immune cells, such as myeloid-derived suppressor cells (MDSCs), populate inflamed or cancerous tissue and block immune cell effector functions. The lack of mechanistic insight into MDSC suppressive activity and a marker for their identification has hampered attempts to overcome T cell inhibition and unleash anti-cancer immunity. Here, we report that human MDSCs were characterized by strongly reduced metabolism and conferred this compromised metabolic state to CD8+ T cells, thereby paralyzing their effector functions. We identified accumulation of the dicarbonyl radical methylglyoxal, generated by semicarbazide-sensitive amine oxidase, to cause the metabolic phenotype of MDSCs and MDSC-mediated paralysis of CD8+ T cells. In a murine cancer model, neutralization of dicarbonyl activity overcame MDSC-mediated T cell suppression and, together with checkpoint inhibition, improved the efficacy of cancer immune therapy. Our results identify the dicarbonyl methylglyoxal as a marker metabolite for MDSCs that mediates T cell paralysis and can serve as a target to improve cancer immune therapy.Entities:
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Year: 2020 PMID: 32327756 DOI: 10.1038/s41590-020-0666-9
Source DB: PubMed Journal: Nat Immunol ISSN: 1529-2908 Impact factor: 25.606