Isotope tracing reveals distinct substrate preference in murine melanoma subtypes with differing anti-tumor immunity

Xinyi Zhang; Alexandra A Halberstam; Wanling Zhu; Brooks P Leitner; Durga Thakral; Marcus W Bosenberg; Rachel J Perry

doi:10.1186/s40170-022-00296-7

Isotope tracing reveals distinct substrate preference in murine melanoma subtypes with differing anti-tumor immunity

Cancer Metab. 2022 Dec 1;10(1):21. doi: 10.1186/s40170-022-00296-7.

Authors

Xinyi Zhang^{1

2}, Alexandra A Halberstam^{1

2}, Wanling Zhu^{1

2}, Brooks P Leitner^{1

2}, Durga Thakral³, Marcus W Bosenberg^{3

4

5

6

7

8}, Rachel J Perry^{9

10}

Affiliations

¹ Department of Internal Medicine (Endocrinology), Yale School of Medicine, P.O. Box 208026, 333 Cedar St., SHM BE36-B, New Haven, CT, 06520-8026, USA.
² Department of Cellular & Molecular Physiology, Yale School of Medicine, New Haven, USA.
³ Department of Pathology, Yale School of Medicine, New Haven, USA.
⁴ Department of Dermatology, Yale School of Medicine, New Haven, USA.
⁵ Department of Immunobiology, Yale School of Medicine, New Haven, CT, USA.
⁶ Yale Stem Cell Center, New Haven, CT, USA.
⁷ Yale Cancer Center, New Haven, CT, USA.
⁸ Yale Center for Immuno-Oncology, New Haven, CT, USA.
⁹ Department of Internal Medicine (Endocrinology), Yale School of Medicine, P.O. Box 208026, 333 Cedar St., SHM BE36-B, New Haven, CT, 06520-8026, USA. rachel.perry@yale.edu.
¹⁰ Department of Cellular & Molecular Physiology, Yale School of Medicine, New Haven, USA. rachel.perry@yale.edu.

Abstract

Background: Research about tumor "metabolic flexibility"-the ability of cells to toggle between preferred nutrients depending on the metabolic context-has largely focused on obesity-associated cancers. However, increasing evidence for a key role for nutrient competition in the tumor microenvironment, as well as for substrate regulation of immune function, suggests that substrate metabolism deserves reconsideration in immunogenic tumors that are not strongly associated with obesity.

Methods: We compare two murine models: immunologically cold YUMM1.7 and immunologically-hot YUMMER1.7. We utilize stable isotope and radioisotope tracer-based metabolic flux studies as well as gas and liquid chromatography-based metabolomics analyses to comprehensively probe substrate preference in YUMM1.7 and YUMMER1.7 cells, with a subset of studies on the impact of available metabolites across a panel of five additional melanoma cell lines. We analyze bulk RNA-seq data and identify increased expression of amino acid and glucose metabolism genes in YUMMER1.7. Finally, we analyze melanoma patient RNA-seq data to identify potential prognostic predictors rooted in metabolism.

Results: We demonstrate using stable isotope tracer-based metabolic flux studies as well as gas and liquid chromatography-based metabolomics that immunologically-hot melanoma utilizes more glutamine than immunologically-cold melanoma in vivo and in vitro. Analyses of human melanoma RNA-seq data demonstrate that glutamine transporter and other anaplerotic gene expression positively correlates with lymphocyte infiltration and function.

Conclusions: Here, we highlight the importance of understanding metabolism in non-obesity-associated cancers, such as melanoma. This work advances the understanding of the correlation between metabolism and immunogenicity in the tumor microenvironment and provides evidence supporting metabolic gene expression as potential prognostic factors of melanoma progression and may inform investigations of adjunctive metabolic therapy in melanoma.

Trial registration: Deidentified data from The Cancer Genome Atlas were analyzed.

Keywords: Amino acid; Glucose; Melanoma; Tumor metabolism; Tumor microenvironment.

Abstract

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